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<script type="text/javascript" src="/corehtml/pmc/jatsreader/ptpmc_3.22/js/jr.boots.min.js"> </script><title>Glycosylation Engineering - Essentials of Glycobiology - NCBI Bookshelf</title>
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<meta name="citation_inbook_title" content="Essentials of Glycobiology [Internet]. 3rd edition">
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<meta name="citation_title" content="Glycosylation Engineering">
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<meta name="citation_publisher" content="Cold Spring Harbor Laboratory Press">
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<meta name="citation_date" content="2017">
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<meta name="citation_author" content="Henrik Clausen">
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<meta name="citation_author" content="Hans H. Wandall">
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<meta name="citation_author" content="Catharina Steentoft">
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<meta name="citation_author" content="Pamela Stanley">
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<meta name="citation_author" content="Ronald L. Schnaar">
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<meta name="citation_doi" content="10.1101/glycobiology.3e.056">
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<meta name="DC.Title" content="Glycosylation Engineering">
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<meta name="DC.Contributor" content="Henrik Clausen">
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<meta name="DC.Contributor" content="Hans H. Wandall">
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<meta name="DC.Contributor" content="Catharina Steentoft">
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<meta name="DC.Contributor" content="Pamela Stanley">
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<meta name="DC.Contributor" content="Ronald L. Schnaar">
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<meta name="og:description" content="Knowledge of the cellular pathways of glycosylation across phylogeny provides opportunities for designing glycans via genetic engineering in a wide variety of cell types including bacteria, fungi, plant cells, and mammalian cells. The commercial demand for glycosylation engineering is broad, including production of biological therapeutics with defined glycosylation (Chapter 57). This chapter describes how knowledge of glycan structures and their metabolism (Parts I–III of this book) has led to the current state of glycosylation engineering in different cell types. Perspectives for rapid advances in this area using precise gene editing technologies are also described.">
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next match">▶</a></nav></nav></div><div id="jr-epub-interstitial" class="hidden"></div><div id="jr-content"><article data-type="main"><p class="vip-notice"><strong><a href="/books/n/glyco4/?report=reader">A new version of this title is available</a></strong></p><p class="vip-notice"><strong><a href="/books/NBK579915/?report=reader">See the updated version of this chapter</a></strong></p><div class="main-content lit-style" itemscope="itemscope" itemtype="http://schema.org/CreativeWork"><div class="meta-content fm-sec"><div class="fm-sec"><h1 id="_NBK453027_"><span class="label">Chapter 56</span><span class="title" itemprop="name">Glycosylation Engineering</span></h1><p class="contribs">Clausen H, Wandall HH, Steentoft C, et al.</p><p class="fm-aai"><a href="#_NBK453027_pubdet_">Publication Details</a></p></div></div><div class="jig-ncbiinpagenav body-content whole_rhythm" data-jigconfig="allHeadingLevels: ['h2'],smoothScroll: false" itemprop="text"><div id="_abs_rndgid_" itemprop="description"><p>Knowledge of the cellular pathways of glycosylation across phylogeny provides opportunities for designing glycans via genetic engineering in a wide variety of cell types including bacteria, fungi, plant cells, and mammalian cells. The commercial demand for glycosylation engineering is broad, including production of biological therapeutics with defined glycosylation (<a href="/books/n/glyco3/ch57/?report=reader">Chapter 57</a>). This chapter describes how knowledge of glycan structures and their metabolism (Parts I–III of this book) has led to the current state of glycosylation engineering in different cell types. Perspectives for rapid advances in this area using precise gene editing technologies are also described.</p></div><div id="Ch56_s1"><h2 id="_Ch56_s1_">GOALS FOR GLYCOENGINEERING OF CELLS</h2><p>There is a long history of engineering glycosylation in mammalian cells, plants, fungi (yeast), and bacteria using genetic strategies, and many well-characterized glycosylation mutants are available (<a href="/books/n/glyco3/ch20/?report=reader">Chapters 20</a>–<a href="/books/n/glyco3/ch27/?report=reader">27</a> and <a href="/books/n/glyco3/ch49/?report=reader">49</a>). Today, cellular glycoengineering is used extensively to produce recombinant therapeutic glycoproteins that require glycosylation for their efficacy and at the same time must have human-compatible glycosylation to avoid immune responses to nonhuman glycans. Glycosylation can alter the size, charge, and solubility of therapeutic glycoproteins to prevent rapid clearance from the circulation. In addition, glycoengineering has been used to improve or develop new therapeutic modalities (<a href="/books/n/glyco3/ch57/?report=reader">Chapter 57</a>). Glycans can also serve as ligands for lectin receptors that target therapeutics to certain cells. Of particular importance is the role of N-glycosylation for effector functions of IgG antibodies; therapeutic IgG antibodies with N-glycosylation designed to improve their cytotoxic properties are in clinical use. In the past decade, new methods have emerged to precisely engineer glycosylation by gene editing, and with increased knowledge the field seems to be limited only by imagination.</p><p>Cell lines are widely used as factories to produce recombinant glycoproteins from introduced gene constructs. The most common factories for glycoproteins include yeast, plants, insect cells, nonhuman mammalian cells, and more rarely human cells. More recently, bacteria are also being engineered to accommodate production of glycoproteins. The glycosylation capabilities of different species vary substantially in terms of both the sites of glycan attachment and the glycans attached (<a class="figpopup" href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" rid-figpopup="figch56f1" rid-ob="figobch56f1">Figure 56.1</a> and <a href="/books/n/glyco3/ch9/?report=reader">Chapters 9</a>–<a href="/books/n/glyco3/ch27/?report=reader">27</a>). A first step in glycoengineering strategies is therefore to consider which cell type to use. This decision requires detailed knowledge of glycosylation pathways and genes. Historically, the mammalian Chinese hamster ovary (CHO) cell line has played a dominant role, and today most biologics are produced in CHO cells (<a href="/books/n/glyco3/ch49/?report=reader">Chapter 49</a>). The CHO line was selected for human therapeutic production because its glycosylation is relatively simple and similar to that in humans. The CHO cell line produces a comparatively narrow repertoire of glycans; glycoengineering expands their native capabilities and provides for additional optimization of glycoforms. Alternatively, host species in which native glycosylation provides a simpler starting point for engineering can be selected. For example, glycoproteins for enzyme replacement therapies have been produced in yeast and glycan vaccines have been made in bacteria.</p><p>There have been major achievements in glycoengineering of cells from bacteria to yeast and “higher” eukaryotes (<a class="figpopup" href="/books/NBK453027/table/CH56TB1/?report=objectonly" target="object" rid-figpopup="figCH56TB1" rid-ob="figobCH56TB1">Table 56.1</a> and <a href="/books/n/glyco3/ch49/?report=reader">Chapter 49</a>). New precise gene editing technologies described below will enable glycoengineering in a wide variety of species and open opportunities for selection from host cells based on optimal production efficiency and production of human-like glycans. Common principles in glycoengineering via gene editing are described below, followed by more detailed descriptions of progress in cells from various species.</p><div class="iconblock whole_rhythm clearfix ten_col fig" id="figch56f1" co-legend-rid="figlgndch56f1"><a href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" title="FIGURE 56.1." class="img_link icnblk_img figpopup" rid-figpopup="figch56f1" rid-ob="figobch56f1"><img class="small-thumb" src="/books/NBK453027/bin/ch56f01.gif" src-large="/books/NBK453027/bin/ch56f01.jpg" alt="FIGURE 56.1.. Overview of species-specific glycosylation features." /></a><div class="icnblk_cntnt" id="figlgndch56f1"><h4 id="ch56.f1"><a href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" rid-ob="figobch56f1">FIGURE 56.1.</a></h4><p class="float-caption no_bottom_margin">Overview of species-specific glycosylation features. The figure presents the different classes of glycoconjugates present in mammalian, plant, insect, and yeast cells with a representative glycan from each class. Structures to the right of the break are <a href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" rid-ob="figobch56f1">(more...)</a></p></div></div><div class="iconblock whole_rhythm clearfix ten_col table-wrap" id="figCH56TB1"><a href="/books/NBK453027/table/CH56TB1/?report=objectonly" target="object" title="TABLE 56.1." class="img_link icnblk_img figpopup" rid-figpopup="figCH56TB1" rid-ob="figobCH56TB1"><img class="small-thumb" src="/books/NBK453027/table/CH56TB1/?report=thumb" src-large="/books/NBK453027/table/CH56TB1/?report=previmg" alt="TABLE 56.1." /></a><div class="icnblk_cntnt"><h4 id="CH56TB1"><a href="/books/NBK453027/table/CH56TB1/?report=objectonly" target="object" rid-ob="figobCH56TB1">TABLE 56.1.</a></h4><p class="float-caption no_bottom_margin">Examples of major achievements in glycoengineering of cells </p></div></div></div><div id="Ch56_s2"><h2 id="_Ch56_s2_">KNOWLEDGE OF GLYCOSYLATION PATHWAYS ENABLES GLYCOENGINEERING</h2><p>Although the glycomes of different species have distinct features (<a class="figpopup" href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" rid-figpopup="figch56f1" rid-ob="figobch56f1">Figure 56.1</a>), the basic biosynthetic machinery and pathways are remarkably conserved in eukaryotes, and there are even similarities with glycosylation pathways in some bacteria and archaea. Most enzymes involved in glycosylation in eukaryotes are highly conserved in fungi, plants, and animals facilitating the design and execution of glycoengineering strategies in these organisms. Nevertheless, current knowledge is far from complete and glycoengineering across species is still in its infancy. Whereas expression of a particular protein in a heterologous host may require only introduction of the single gene for that protein, precise glycosylation engineering of that protein may require cointroduction of a suite of genes including those required for the biosynthesis and transport of appropriate activated nucleotide sugar donors as well as multiple glycosyltransferases.</p><p>Successful glycoengineering requires knowledge of the glycosyltransferase genes and substrates required to direct synthesis of a particular glycan. Certain genes may need to be removed and others inserted to create biosynthetic pathways that produce the glycans of interest. Three decades of glycogene discoveries have resulted in the identification of most genes encoding glycosyltransferases, hydrolases, and other enzymes involved in synthesizing and metabolizing the glycans of “higher” eukaryotic cells and the “rules” of the biosynthetic pathways involved (<a href="/books/n/glyco3/ch8/?report=reader">Chapters 8</a>–<a href="/books/n/glyco3/ch19/?report=reader">19</a>). Different glycosylation pathways may be performed independently by different sets of enzymes, or in some cases, may share enzymes. Enzymes working in consecutive order to assemble mature glycans generally work independently, although there may also be cooperative effects. In principle, there is sufficient knowledge to predict the role of individual enzymes and assign them to specific pathways, allowing in silico prediction of the enzyme repertoire required to generate a particular glycan on a particular glycoconjugate. An excellent resource in this regard is the classification of homologous gene families from diverse species in the “Carbohydrate-Active Enzymes” (<a href="http://www.cazy.org/" ref="pagearea=body&targetsite=external&targetcat=link&targettype=uri">CAZy</a>) database (<a href="/books/n/glyco3/ch8/?report=reader">Chapter 8</a>).</p><p>Among the prerequisites for glycoengineering a desired glycan in a chosen host is that the appropriate repertoire of activated sugar donors and their transporters are present (<a href="/books/n/glyco3/ch5/?report=reader">Chapter 5</a>). This is especially important when engineering glycosylation in prokaryotes or nonmammalian eukaryotes in which the nucleotide sugar donors required to synthesize therapeutics with human glycosylation may not be present. For example, yeast and plants do not produce UDP-GalNAc, and many organisms do not produce CMP-sialic acids.</p></div><div id="Ch56_s3"><h2 id="_Ch56_s3_">THE IN/OUT STRATEGIES OF GENETIC GLYCOENGINEERING</h2><p>Different genetic strategies may be used to alter the glycosylation capabilities of cells. Knockdown and nontargeted overexpression have been used for many years, although precisely targeted gene editing strategies have only recently been introduced.</p><div id="Ch56_s3a"><h3>Knockdown</h3><p>Reducing undesirable glycosyltransferase activities in cells has been achieved by gene silencing strategies. Whereas this has been particularly successful in plants and Drosophila, silencing has not gained wide use in glycoengineering mammalian cell lines because the low efficiency of knockdown often leaves substantial glycosyltransferase activity remaining.</p></div><div id="Ch56_s3b"><h3>Overexpression</h3><p>Adding desirable glycosyltransferase activities is achieved by transfection of glycogenes from any organism, random integration of plasmid DNA and antibiotic selection of stable clones. Although this strategy is successful, it provides little control over site(s) of genomic integration, gene copy number, or gene expression levels. Overexpression of enzymes can lead to disruption of normal glycosylation patterns and unpredictable glycosylation. Instability of the introduced glycosylation traits and the use of antibiotics for selection have also been problematic for the long-term use of such engineered cells for production of therapeutic glycoproteins.</p></div><div id="Ch56_s3c"><h3>Knockout and Knockin by Precision Genome Editing</h3><p>Knockout of glycosylation genes to eliminate unwanted glycans has long been a simple task in bacteria and yeast. Although powerful, knockout or knockin strategies have been time consuming and difficult to use in “higher” eukaryotic cells (consider the <i>Fut8</i> knockout in CHO cells described below), these difficulties were substantially reduced with the introduction of nuclease-based precise gene editing tools including zinc-finger nucleases, transcription activator–like effector nucleases (TALENs), and clustered regularly interspaced short palindromic repeat/targeted Cas9 endonuclease (CRISPR/Cas9), which enable highly specific gene manipulation in all cell types (<a class="figpopup" href="/books/NBK453027/figure/ch56.f2/?report=objectonly" target="object" rid-figpopup="figch56f2" rid-ob="figobch56f2">Figure 56.2</a>; <a href="/books/n/glyco3/ch27/?report=reader">Chapters 27</a> and <a href="/books/n/glyco3/ch49/?report=reader">49</a>). Importantly, these tools are not limited to gene knockout or knockin but can also be used to activate endogenous silent genes, edit gene sequences to mimic hypomorphic disease mutations, and insert foreign genes at specific genomic sites.</p><div class="iconblock whole_rhythm clearfix ten_col fig" id="figch56f2" co-legend-rid="figlgndch56f2"><a href="/books/NBK453027/figure/ch56.f2/?report=objectonly" target="object" title="FIGURE 56.2." class="img_link icnblk_img figpopup" rid-figpopup="figch56f2" rid-ob="figobch56f2"><img class="small-thumb" src="/books/NBK453027/bin/ch56f02.gif" src-large="/books/NBK453027/bin/ch56f02.jpg" alt="FIGURE 56.2.. Precise gene editing modalities." /></a><div class="icnblk_cntnt" id="figlgndch56f2"><h4 id="ch56.f2"><a href="/books/NBK453027/figure/ch56.f2/?report=objectonly" target="object" rid-ob="figobch56f2">FIGURE 56.2.</a></h4><p class="float-caption no_bottom_margin">Precise gene editing modalities. Glycosyltransferases are represented with their catalytic domains and amino-terminal membrane spanning domains. Examples of gene edition for gene disruption (knockout), editing (mutation), tagging, and insertion of heterologous <a href="/books/NBK453027/figure/ch56.f2/?report=objectonly" target="object" rid-ob="figobch56f2">(more...)</a></p></div></div><p>Precise gene editing can insert foreign genes at “safe harbor” sites in the genome to ensure stable expression and avoid interfering with endogenous gene expression. One such “safe harbor” in human cells is the AAVS1 site on chromosome 19 known to enable stable expression of transgenes without adverse effects. However, precise genetic engineering allows insertion of one or more foreign genes at any position in the genome. For example, precise knockin of glycogenes can be combined with knockout by inserting an exogenous gene in place of an unwanted endogenous gene. Precise knockin strategies also enable control of the number of copies inserted, and can be used to insert entire landing platforms of multiple genes inserted consecutively.</p><p>Successful expression of an enzyme or transporter for glycoengineering requires that the expressed protein finds its way to the correct subcellular compartment. Heterologous expression of type 2 Golgi transmembrane glycosyltransferases, for example, often requires testing different Golgi retention sequences. Although design guidance is available, this is often a trial and error exercise, and in some cases a combinatorial screening is required to identify the optimal construct.</p></div></div><div id="Ch56_s4"><h2 id="_Ch56_s4_">GLYCOENGINEERING IN BACTERIA</h2><p>The most common bacterium used for heterologous protein production, <i>Escherichia coli</i>, does not have the native capacity to glycosylate proteins. However, research in the last two decades identified N- and O-glycoproteins, and the glycosylation pathways responsible for their biosynthesis, in the pathogenic proteobacterium <i>Campylobacter jejuni</i> and other bacterial species. Moreover, several bacterial toxins have glycosyltransferase domains that exert their pathogenicity by glycosylating highly specific amino acids in key host proteins to interfere with essential cellular functions. <a href="/books/n/glyco3/ch21/?report=reader">Chapter 21</a> discusses glycosylation in Eubacteria. Another unique feature of bacteria is that sugar nucleotide donors are synthesized and remain in the cytosol, so that engineered glycosylation must take place in the cytosol unless nucleotide sugar transporters are introduced.</p><div id="Ch56_s4a"><h3>Engineering Free and Lipid-Linked Oligosaccharides</h3><p>Bacteria efficiently produce free and lipid-linked oligo- and polysaccharides including capsular polysaccharides (CPSs) and lipopolysaccharides (LPSs) (<a href="/books/n/glyco3/ch21/?report=reader">Chapter 21</a>), and these pathways have been engineered to produce a variety of complex human-like glycans. In particular, the LPS pathway has been used to engineer and display glycans in <i>E. coli</i>. LPS consists of a base lipid (lipid A) linked to a core oligosaccharide followed by highly diverse O-polysaccharides (O-antigens). Genetically interrupting biosynthesis of the lipid A core oligosaccharide prevents coupling of the O-antigen, instead allowing engineering of novel glycans on lipid A for display on the cell surface. This strategy has been used to engineer the synthesis of a variety of human glycan epitopes, including blood group antigens and cancer-associated glycolipid glycans.</p></div><div id="Ch56_s4b"><h3>Engineering N-Glycosylation</h3><p>Two types of native protein N-glycosylation occur in some bacteria, although not in <i>E. coli</i>. One type is similar to eukaryotic cell N-glycosylation with production of a lipid-linked oligosaccharide in the cytosol which is then transferred en bloc to Asn residues by an oligosaccharyltransferase (OST) in the periplasm. The OST of <i>C. jejuni</i>, PglB, is a single polypeptide related to the catalytic STT3 subunits of the multiprotein OST complex of eukaryotes. PglB shows a more restricted acceptor sequence motif than the eukaryotic N-X-S/T, with requirement of an acidic residue (D/EXNXS/T, in which X cannot be P) (<a href="/books/n/glyco3/ch21/?report=reader">Chapter 21</a>). This places some restrictions on the usefulness of engineering human-like N-glycans, because most N-glycan sites in mammalian proteins do not conform to this extended consensus sequence. PglBs from other species or mutants evolved by adaptive evolution may solve this problem in the future. Importantly, PglB has rather relaxed donor substrate specificity. Although bacterial lipid-linked oligosaccharides are distinct from those in eukaryotes, PglB can use mammalian type lipid-linked oligosaccharides as donors.</p><p>An important feature for using prokaryotes for glycoengineering is the arrangement of entire glycosylation machineries in multigene operons. This enables the transfer of large genetic elements of 10–20 kb between species. A major achievement was the successful transfer of the entire N-glycosylation operon from <i>C. jejuni</i> to <i>E. coli</i>, producing N-linked glycoproteins in <i>E. coli</i> (<a class="figpopup" href="/books/NBK453027/table/CH56TB1/?report=objectonly" target="object" rid-figpopup="figCH56TB1" rid-ob="figobCH56TB1">Table 56.1</a>). Production of glycoproteins carrying a Man<sub>3</sub>GlcNAc<sub>2</sub> core N-glycan has been achieved by introduction of eukaryotic enzymes, and the engineering of more complex glycans may be possible. Bacterial N-linked glycosylation is being exploited as an alternative method for glycoconjugate vaccine production, and vaccines against both Gram-negative and Gram-positive bacteria have been developed.</p><p>Another type of N-glycosylation found in γ-proteobacteria involves a cytosolic N-glycosyltransferase (NGT) that targets the N-X-S/T acceptor sequence motif recognized by mammalian OST (<a href="/books/n/glyco3/ch9/?report=reader">Chapter 9</a>). NGT transfers a single monosaccharide (e.g., Glc) from an activated sugar nucleotide donor, with loose donor substrate specificity that includes both UDP and GDP sugar nucleotides. This provides an entirely new approach to engineering N-glycosylation with a wide array of glycans that cannot be engineered in eukaryotic cells. Although further engineering of this pathway in bacteria has not been reported, attached Glc residues in glycoproteins have been used for postexpression conjugation of mammalian-type oligosaccharides.</p><p>A limitation of bacteria for glycoengineering is that most bacteria do not have the capacity for sialylation and do not synthesize CMP-sialic acid. To introduce sialylation, it is necessary to insert the entire sialylation pathway as has been performed in other organisms. However, some bacteria do sialylate lipid-linked oligosaccharides using sialyltransferases with specificities similar to some of those in mammals.</p></div><div id="Ch56_s4c"><h3>Engineering O-Glycosylation</h3><p>Protein O-glycosylation in bacteria is unlike the stepwise biosynthesis of O-glycans in eukaryotes (<a href="/books/n/glyco3/ch10/?report=reader">Chapter 10</a>), in that preassembled undecaprenol-PP-linked oligosaccharides are transferred en bloc to proteins by several OSTs (<i>PglL</i>, <i>PilO</i>, <i>PglA</i>, and <i>PglO</i>) with relaxed donor substrate specificities and poorly understood acceptor substrate specificities. Bacteria may also have OST–independent O-glycosylation pathways controlled by glycosyltransferases using activated sugar donors. Although engineering of the endogenous O-glycosylation machinery of bacteria has not been performed, human O-glycosylation has been engineered into <i>E. coli</i> by introducing mammalian polypeptide GalNAc-transferase genes and a UDP-Glc/GlcNAc C4-epimerase to produce O-GalNAc glycosylation. Site-specific introduction of GalNAc residues has been used for postexpression enzymatic addition of polyethylene glycol (PEG)-derivatized sialic acids to enhance the therapeutic properties of protein drugs.</p></div></div><div id="Ch56_s5"><h2 id="_Ch56_s5_">GLYCOENGINEERING IN YEAST</h2><p>Yeast natively produce N-linked glycans and O-mannosyl glycans on diverse glycoproteins. The general features of the biosynthetic pathways for initial glycan transfer are common in eukaryotes from yeast to human, and the enzymes involved are highly homologous. However, subsequent glycan processing in yeast generally results in polymannosylated glycans instead of the complex N- and O-glycans found in “higher” eukaryotes (<a class="figpopup" href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" rid-figpopup="figch56f1" rid-ob="figobch56f1">Figure 56.1</a>). Yeast have similar systems for protein folding, quality control, and posttranslational modifications to “higher” eukaryotic cells, in contrast to bacteria. Because genetic engineering in yeast has long been rapid and easy, experience with glycoengineering is more advanced in this organism compared with most others. Several commercial ventures have been based on engineering “humanized” N-glycosylation in yeast; GlycoFi Inc. claimed to have engineered yeast expressing biantennary N-glycans capped by sialic acids, but many years have passed without commercial application. Independently, a related engineering strategy that also eliminates Man-P modifications of N-glycans has been developed (GlycoSwitch).</p><div id="Ch56_s5a"><h3>Engineering N-Glycosylation</h3><p>N-glycans on yeast glycoproteins differ from those in vertebrates (<a href="/books/n/glyco3/ch9/?report=reader">Chapter 9</a>), comprising large polymannosyl glycans on a poly(Manα1-6)<sub>n</sub> backbone which are highly immunogenic in mammals (<a href="/books/n/glyco3/ch23/?report=reader">Chapter 23</a>). A key α1-6-mannosyltransferase, Och1p largely initiates polymannosylation. Knockout of the <i>OCH1</i> gene, however, does not completely abrogate polymannosylation and additional knockout of mannosyl- and phosphomannosyltransferases, dependent on yeast strain, are needed to achieve a homogenous Man<sub>8</sub>GlcNAc<sub>2</sub> N-glycan suitable for further engineering. Reducing Man<sub>8</sub>GlcNAc<sub>2</sub> to Man<sub>5</sub>GlcNAc<sub>2</sub> is achieved by expressing an α1-2–mannosidase in the endoplasmic reticulum (ER), creating a convenient platform for generating complex N-glycans. Introduction of GlcNAcT-I (<i>MGAT1</i>) in the Golgi initiates complex N-glycan synthesis, and further addition of α3/6-mannosidase II (<i>MAN2A1</i>) and GlcNAcT-II (<i>MGAT2</i>) results in the biantennary GlcNAc<sub>2</sub>Man<sub>3</sub>GlcNAc<sub>2</sub> N-glycan suitable for appending galactosylation and sialylation by further engineering. Some yeast species, including <i>Pichia pastoris</i>, do not contain UDP-Gal, and all yeast lack the native ability to synthesize CMP-Neu5Ac, so considerable engineering with introduction of multiple genes is required to obtain mature complex N-glycans. Although the engineering appears simple in silico, considerable efforts have been devoted to identifying optimal chimeric gene constructs with respect to both catalytic efficiency and ER/Golgi targeting.</p></div><div id="Ch56_s5b"><h3>Engineering O-Glycosylation</h3><p>Yeast performs extensive co- and posttranslational ER protein O-mannosylation (<a href="/books/n/glyco3/ch23/?report=reader">Chapter 23</a>) using several polypeptide mannosyltransferases (PMTs). <i>Saccharomyces cerevisiae</i> has six PMTs and only a subset can be knocked out without reducing viability. Protein O-Man residues undergo polymannosylation in the Golgi. “Higher” eukaryotes also perform O-mannosylation and express two PMT orthologs, <i>POMT1</i> and <i>POMT2</i> (<a href="/books/n/glyco3/ch13/?report=reader">Chapter 13</a>), but these have much narrower acceptor substrate specificities. However, “higher” eukaryotes perform several other types of O-glycosylation (<a class="figpopup" href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" rid-figpopup="figch56f1" rid-ob="figobch56f1">Figure 56.1</a>) (<a href="/books/n/glyco3/ch10/?report=reader">Chapters 10</a>, <a href="/books/n/glyco3/ch13/?report=reader">13</a>, and <a href="/books/n/glyco3/ch14/?report=reader">14</a>), and their O-GalNAc glycans tend to be located in similar regions and protein sites as O-Man glycans in yeast. This means that expression of human O-glycoproteins in yeast may result in O-mannosylation at sites that carry O-GalNAc in mammals. Examples of this include the hinge region of IgA and mucin sequences. Because it is still difficult to predict types of O-glycosylation, human proteins expressed in yeast must be tested to determine if they are O-mannosylated.</p><p>Human O-GalNAc glycans have been successfully engineered into yeast by introducing human protein GalNAc transferases along with UDP-Glc/GlcNAc C4-epimerase and a UDP-Gal/GalNAc Golgi transporter. The entire biosynthetic machinery for CMP-Neu5Ac synthesis and transport has also been introduced together with a human sialyltransferase, and sialylated O-glycans have been produced in yeast. The problem with competing endogenous O-mannosylation can be partly eliminated by including a mannosyltransferase inhibitor (rhodanine-3-acetic acid). A deeper understanding of the yeast O-Man and human O-GalNAc glycosylation pathways is needed to provide new strategies to circumvent competition between the two systems and enhance O-glycan engineering in yeast.</p></div></div><div id="Ch56_s6"><h2 id="_Ch56_s6_">GLYCOENGINEERING IN PLANT CELLS</h2><p>Plants offer a simpler starting point than yeast for N-glycan humanization because the predominant native N-glycans of plants are paucimannose (Man<sub>3</sub>GlcNAc<sub>2</sub>) and biantennary terminating in GlcNAc (GlcNAc<sub>2</sub>Man<sub>3</sub>GlcNAc<sub>2</sub>). The abundance of paucimannose N-glycans appears to be due to a β-hexosaminidase that removes attached GlcNAc residues in competition with GlcNAc-transferases, a feature also found in insect cells. Two plant-specific N-glycan modifications include core α1-3-Fuc (instead of mammalian core α1-6-Fuc) and β1-2-Xyl linked to the β-Man in the N-glycan core. Both modifications are potentially immunogenic in humans. Plants also produce unique types of O-glycosylation not found in other species that pose potential problems for the generation of therapeutic glycoproteins.</p><div id="Ch56_s6a"><h3>Engineering N-Glycosylation</h3><p>Great advances in engineering plants for human-like N-glycosylation have been achieved. Knockdown or knockout of the β-hexosaminidase that inhibits complex N-glycan formation, as well as the α1-3-fucosyltransferase and β1-2-xylosyltransferase, have been achieved in different plants, including <i>Arabidopsis thaliana</i> and <i>Nicotiana benthamiana</i>. Nearly homogeneous biantennary GlcNAc<sub>2</sub>Man<sub>3</sub>GlcNAc<sub>2</sub> N-glycans were produced. These were further engineered by the introduction of Gal (using <i>B4GALT1</i>) and sialic acid (using <i>ST6GAL1</i> along with the enzymes needed to synthesize and transport CMP-Neu5Ac) in an engineering design using up to six gene constructs. Such humanized plants produced α2-6-Neu5Ac capped biantennary N-glycans without core fucose on a variety of recombinant glycoproteins. These achievements depended on combinatorial screening strategies to identify appropriate chimeric constructs of exogenous enzymes to drive the engineered glycosylation toward homogeneity.</p><p>Glycoproteins produced in plants carrying native paucimannose N-glycosylation are already in use as approved drugs. For enzyme replacement therapy, the terminal mannose N-glycans of glucocerebrosidase (taliglucerase alfa) produced in carrots is beneficial for targeting to endogenous human mannose receptors, despite α1-3-Fuc and β1-2-Xyl modifications, and is in clinical use. Moreover, glycoengineered <i>Nicotiana bethamiana</i> cells without α1-3-Fuc and β1-2-Xyl have been used to produce a triple antibody cocktail used to treat Ebola virus infections.</p></div><div id="Ch56_s6b"><h3>Engineering O-Glycosylation</h3><p>Plants do not have the types of O-glycosylation found in other eukaryotes, but produce extensins and arabinogalactan proteins with two unique O-glycans. A family of prolyl-4-hydroxylases (P4H) converts selected Pro residues to hydroxyproline that may be arabinosylated by a series of enzymes. In addition, Ser residues may be O-glycosylated by the addition of Gal residues. Although a number of the P4Hs and glycosyltransferases have been knocked out in different plants, it is unclear whether these modifications can be completely eliminated without affecting viability. Nonetheless, the human machinery for O-GalNAc glycosylation has been engineered into plants. Similar to bacteria and yeast, this involves introducing an UDP-Glc/GlcNAc C4-epimerase as well as the necessary polypeptide GalNAc transferases, but a dedicated UDP-GalNAc transporter is not required. Human core 1 glycosylation, as well as the complete sialylation machinery with a ST3GALI sialyltransferase have also been successfully introduced in plants. If issues related to hydroxyproline can be resolved, plants offer a valuable system in which different types of mammalian O-glycosylation can be engineered and exploited. A clear highlight of glycoengineering in plants is the combined introduction of 14 genes for production of the major human therapeutic glycoprotein erythropoietin with human sialylated biantennary N-glycans and core 1 O-glycans in tobacco cells (<a class="figpopup" href="/books/NBK453027/table/CH56TB1/?report=objectonly" target="object" rid-figpopup="figCH56TB1" rid-ob="figobCH56TB1">Table 56.1</a>).</p></div></div><div id="Ch56_s7"><h2 id="_Ch56_s7_">GLYCOENGINEERING IN INSECT CELLS</h2><p>Engineering in insect cells involves multiple strategies. Two different platforms are generally used for recombinant expression of proteins—transient expression in baculovirus and stable expression in S2 <i>Drosophila melanogaster</i> cells. For the baculovirus expression platform, glycoengineering may be achieved by including glycosylation genes with the recombinant baculovirus vector, or introduced in the insect cell line used for infection and expression. Stable engineering of host insect cell lines may be the most efficient and consistent strategy, but remarkable success has been achieved by incorporating up to nine glycogenes in a baculovirus vector (<a class="figpopup" href="/books/NBK453027/table/CH56TB1/?report=objectonly" target="object" rid-figpopup="figCH56TB1" rid-ob="figobCH56TB1">Table 56.1</a>). Nevertheless, it is anticipated that only stable engineering of the host cells will eventually enable efficient production of homogeneous glycoforms.</p><div id="Ch56_s7a"><h3>Engineering N-Glycosylation</h3><p>Insect cells produce mostly paucimannose N-glycans despite their enzymatic ability to produce complex galactosylated N-glycans (<a class="figpopup" href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" rid-figpopup="figch56f1" rid-ob="figobch56f1">Figure 56.1</a>). This is primarily due to a highly efficient β-hexosaminidase, FDL, which removes attached GlcNAc residues from the α1-3-Man branch, but it is probably also because insect cells appear to express low <i>MGAT2</i> activity. Like plants, insects also add the potential immunogenic core α1-3–Fuc and do not typically perform sialylation. This has been addressed by introducing sialic acid synthase, CMP-sialic acid synthase, and an <i>N</i>-acetylglucosamine-6-phosphate 2′-epimerase into insect cells. For efficient sialylation, a dedicated CMP-sialic acid transporter appears to be needed as well. Using different strategies, production of glycoproteins carrying biantennary N-glycans with galactosylation and sialic acid capping has been achieved. However, RNAi silencing strategies targeting FDL and the α1-3-fucosyltransferase have been somewhat ineffective, and efficient formation of complex N-glycans has not yet been achieved. Recently, precision gene editing was used to knock out FDL in Sf9 cells, showing the usage of this technology for insect cell engineering.</p></div><div id="Ch56_s7b"><h3>Engineering O-Glycosylation</h3><p>Insect cells perform the same range of O-glycosylation as mammalian cells (<a class="figpopup" href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" rid-figpopup="figch56f1" rid-ob="figobch56f1">Figure 56.1</a>), although the extent to which O-GalNAc glycans are attached at the same sites as in mammals is unexplored. Moreover, the degree of processing of O-glycans appears incomplete, at least using baculovirus expression. Although insect cells appear to offer a straightforward host for production of glycoproteins with human O-glycans, little has been investigated in this regard.</p></div></div><div id="Ch56_s8"><h2 id="_Ch56_s8_">GLYCOENGINEERING IN MAMMALIAN CELLS</h2><p>The cores of all types of glycoprotein glycans (<a class="figpopup" href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" rid-figpopup="figch56f1" rid-ob="figobch56f1">Figure 56.1</a>) are highly conserved among mammals, although there are terminal glycan variations (<a href="/books/n/glyco3/ch14/?report=reader">Chapter 14</a>). The most popular mammalian cell line used for glycoengineering is the CHO cell line established >50 years ago. The success of the CHO cell line is partly due to the ease with which glycosylation mutants could be isolated (<a href="/books/n/glyco3/ch49/?report=reader">Chapter 49</a>), and it was the first cell used to manufacture a recombinant therapeutic with relatively simple human-type terminal glycans without expression of antigenic nonhuman glycans or unusual modifications of the glycans. As discussed in <a href="/books/n/glyco3/ch49/?report=reader">Chapter 49</a>, the CHO cell line has an important place in glycoengineering history, exemplified by the Lec mutant lines generated by lectin selection. These cell lines with distinct mutations in glycosylation genes have provided tools for the scientific community for more than three decades, and illustrated the importance of access to recombinant proteins with particular glycoforms for discovery of biological functions of glycans. CHO cells can be considered as Glycobiology's gift to Biopharma.</p><p>Major successes have been achieved in engineering CHO and other mammalian cell lines for production of human therapeutics (<a class="figpopup" href="/books/NBK453027/table/CH56TB1/?report=objectonly" target="object" rid-figpopup="figCH56TB1" rid-ob="figobCH56TB1">Table 56.1</a> and <a href="/books/n/glyco3/ch49/?report=reader">Chapters 49</a> and <a href="/books/n/glyco3/ch57/?report=reader">57</a>). The field is, however, undergoing a revolution with the new methods for facile, targeted, precise gene editing that allow the design of almost any conceivable glycosylation capacity in any mammalian cell by combining knockout and knockin events.</p><div id="Ch56_s8a"><h3>Engineering N-Glycosylation</h3><p>The first major feat in gene editing of mammalian cells was elimination of the core α1-6-Fuc for production of recombinant IgG antibodies with enhanced binding to the Fcγ-IIIa receptor (<a class="figpopup" href="/books/NBK453027/table/CH56TB1/?report=objectonly" target="object" rid-figpopup="figCH56TB1" rid-ob="figobCH56TB1">Table 56.1</a>). Overexpression of bisecting GlcNAcT-III (<i>MGAT3</i>) resulted in stable CHO cells with highly limited capacity for core fucosylation (commercialized by Roche). A second strategy involved a tour-de-force approach using homologous recombination to knock out the two <i>FUT8</i> alleles in CHO cells. More than 10,000 CHO clones were screened to identify the final knockout cell (commercialized by BioWa). Although this was an impressive achievement, such laborious random selection limits options for selecting cell clones that retain the attributes needed for optimal bioprocessing. Using precise gene editing the same engineering was rapidly replicated, providing ample clones for selection of those with optimal properties. Glycoengineered CHO lines optimized for antibody production are now commercially available (Potelligent CHOK1SV, Lonza/BioWa).</p><p>Engineering N-glycan sialylation has been another focus in the field. CHO cells produce only α2-3-linked sialic acids on N-glycans, whereas human HEK293-T cells (for example) produce a mixture of α2-3- and α2-6-linked sialic acids. Most soluble glycoproteins in human blood (including IgG) have α2-6-linked sialic acids on N-glycans, and reports have suggested that the sialic acid linkage may influence immunomodulatory functions as well as circulatory half-life. It has therefore been of interest to engineer more homogeneous α2-6-sialylation in cells. These efforts have mainly been limited to overexpression of α2-6-siayltransferases to override endogenous α2-3-sialylation with variable results, illustrating the complexity of engineering glycosylation in cells with competing pathways.</p><p>An innovative glycoengineering strategy (GlycoDelete) reduced the inherent heterogeneity of mammalian N-glycan structures. Human HEK293-T cells lacking <i>MGAT1</i> were stably transfected to express a fungal endo-N-acetylglucosaminidase (EndoT) that efficiently truncated N-glycans to a single GlcNAc, which was an acceptor for galactosylation and sialylation. Recombinant antibodies with truncated N-glycans had lower affinity for Fcγ receptors, suggesting that this glycoengineering strategy may be suitable for use with neutralizing antibodies.</p><p>More recently, a fairly complete deconstruction of the N-glycosylation pathway in CHO cells was performed by precise gene editing to knock out 19 glycosyltransferases, including all four α2-3-sialyltransferases that function on N-glycans (<a class="figpopup" href="/books/NBK453027/figure/ch56.f3/?report=objectonly" target="object" rid-figpopup="figch56f3" rid-ob="figobch56f3">Figure 56.3</a>). Combining knockout of <i>St3gal4</i> and <i>St3gal6</i> with site-specific knockin of one copy of <i>St6gal1</i> resulted in homogeneous α2-6-sialylation. Combining combinatorial knockout of all isoenzymes in N-glycan sialylation, galactosylation/LacNAc formation, branching, and core fucosylation has provided a design matrix for improving the homogeneity of N-glycans in CHO cells. A combination of five gene knockouts and the knockin of <i>St6gal1</i> created the glycoprotein therapeutic erythropoietin having homogeneous biantennary N-glycans with terminal α2-6-NeuAc. Although this was an essentially impossible task until recent precise gene editing advances, the strategy can now be applied to any mammalian cell to develop panels of isogenic cell clones with distinct capacities for N-glycosylation.</p><div class="iconblock whole_rhythm clearfix ten_col fig" id="figch56f3" co-legend-rid="figlgndch56f3"><a href="/books/NBK453027/figure/ch56.f3/?report=objectonly" target="object" title="FIGURE 56.3." class="img_link icnblk_img figpopup" rid-figpopup="figch56f3" rid-ob="figobch56f3"><img class="small-thumb" src="/books/NBK453027/bin/ch56f03.gif" src-large="/books/NBK453027/bin/ch56f03.jpg" alt="FIGURE 56.3.. Complex N-glycan with glycosyltransferases responsible for each reaction." /></a><div class="icnblk_cntnt" id="figlgndch56f3"><h4 id="ch56.f3"><a href="/books/NBK453027/figure/ch56.f3/?report=objectonly" target="object" rid-ob="figobch56f3">FIGURE 56.3.</a></h4><p class="float-caption no_bottom_margin">Complex N-glycan with glycosyltransferases responsible for each reaction. Combinatorial knockout of the glycosyltransferase isoenzyme genes indicated led to the identification of the primary genes (highlighted in bold) controlling N-glycan branching (MGATs), <a href="/books/NBK453027/figure/ch56.f3/?report=objectonly" target="object" rid-ob="figobch56f3">(more...)</a></p></div></div><p>Therapeutic glycoprotein production still suffers from heterogeneity, including variations in which Asn residues are glycosylated (site-occupancy, macroheterogeneity) and/or the diversity of mature glycan structures at any one site (microheterogeneity). This is currently addressed by ensuring reproducibility in batch-to-batch production through the use of highly standardized bioprocessing protocols, but this strategy is far from optimal. For example, incompletely sialylated therapeutic glycoproteins may be cleared by the hepatic asialoglycoprotein receptor (Ashwell–Morell receptor), resulting in inconsistent circulatory half-lives of therapeutic glycoproteins. Considerable efforts have been devoted to improving sialylation by overexpressing relevant sialyltransferases as well as inhibiting or knocking out endogenous sialidases in host cells. Protein-specific glycosylation patterns and heterogeneity are more difficult to control.</p><p>Nonhuman mammalian cell lines can produce two immunogenic nonhuman glycans: α1-3-Gal added to <i>N</i>-acetyllactosamine and Neu5Gc added to Gal or GalNAc (<a href="/books/n/glyco3/ch14/?report=reader">Chapters 14</a> and <a href="/books/n/glyco3/ch15/?report=reader">15</a>). The α1-3-galactosyltransferase and CMP-<i>N</i>-acetylneuraminic acid hydrolase genes responsible are inactive in humans. Although α1-3-Gal and Neu5Gc are not produced in CHO cells, both genes have been knocked out as a precaution. Even so, Neu5Gc scavenged from animal glycoproteins used in cell culture can appear in expressed glycoproteins, so use of defined media without nonhuman glycoproteins is also necessary. In engineering mammalian cell lines, it is important to consider that the glycosylation capacity is driven by the expression of a subset of available enzyme genes, but unexpressed genes can become activated. Thus, cell line–specific glycosylation features are generally controlled by transcriptional regulation rather than mutations or gene aberrations. Analysis of all known glycosylation genes in five distinct CHO production cell lines derived from the original CHO-K1 cell line found no apparent deleterious mutations or loss of genes, despite severe chromosomal alterations. This suggests that one must consider all the known glycogenes in a mammalian cell line for glycoengineering strategies.</p><p>Engineering the glycosylation capacity of CHO cells has also enabled more homogeneous bioconjugation of therapeutic drugs. For example, therapeutic drugs may be chemically conjugated with PEG chains to enhance circulatory half-life, but chemical conjugation is difficult to direct to specific sites in glycoproteins. A strategy for enzymatic modification of glycans postproduction has been developed that involves desialylation of recombinant glycoproteins, followed by in vitro transfer of a modified (PEGylated) Neu5Ac (as its CMP analog) to exposed Gal/GalNAc residues by a sialyltransferase. The process is in use with approved drugs, although heterogeneous modifications occur when multiantennary N-glycans are targeted. CHO cells have now been engineered to produce monoantennary, unsialylated N-glycans, which circumvent heterogeneity while retaining multiple exposed Gal acceptor sites for sialo-PEGylation.</p></div><div id="Ch56_s8b"><h3>Engineering O-Glycosylation</h3><p>Mammalian cells perform many different types of O-glycosylation (<a class="figpopup" href="/books/NBK453027/figure/ch56.f1/?report=objectonly" target="object" rid-figpopup="figch56f1" rid-ob="figobch56f1">Figure 56.1</a>), and although these exert diverse and important biological functions, the interest in O-glycans for recombinant therapeutics has been limited. Nevertheless, recombinant coagulation factors in clinical use carry O-GalNAc, O-Fuc, and/or O-Glc glycans, and many other approved drugs including erythropoietin and Enbrel have O-GalNAc glycans. O-glycans are also used for site-specific bioconjugation.</p><p>Engineering O-GalNAc glycans involves a new level of complexity because up to 20 isoenzymes (polypeptide GalNAc-transferases) direct the initiation of O-GalNAc glycans. It may therefore be important to consider the repertoire of these enzymes in a cell line. In theory, a protein that is naturally found with an O-glycan may not be O-glycosylated when expressed in a specific production cell line, and vice versa. Although few examples of this have been identified, an illuminating case is the important phosphaturic factor FGF23, a potential drug for patients with a congenital deficiency associated with hyperphosphatemia which requires an O-GalNAc glycan for activity.</p></div></div><div id="Ch56_s9"><h2 id="_Ch56_s9_">GLYCOENGINEERING IN GLYCOSCIENCE</h2><p>Glycoengineering of cell lines has vast potential to address a number of unmet needs in the glycosciences. As already mentioned, the CHO Lec, Ldl, Pgs, and Pig mutant cell lines (<a href="/books/n/glyco3/ch12/?report=reader">Chapters 12</a> and <a href="/books/n/glyco3/ch49/?report=reader">49</a>) have served the research community for decades by providing defined alterations in glycosylation that enable studies of the functional roles of N-glycans, sialylation, fucosylation, O-glycosylation, proteoglycans, and GPI-anchored proteins. CHO and HEK293-T mutant cells with MGAT1 deficiency have been widely used to produce recombinant proteins with homogeneous N-glycans suitable for crystallization studies.</p><p>Targeted gene editing of whole organisms has provided immense insight into the importance of glycosylation and has revealed biological functions of specific glycosylation genes (<a href="/books/n/glyco3/ch41/?report=reader">Chapter 41</a>). However, discovery of distinct biological functions of specific glycans, and the molecular mechanism(s) involved in multicellular organisms, is complicated by cell-type regulation of glycosylation and the cellular heterogeneity of tissues. Cell lines help to answer certain specific questions and complement whole organism studies.</p><p>Precise gene editing provides vast opportunities for glycoengineering cell lines and designing new strategies to probe glycan functions. Truncation of O-glycan elongation was used to produce homogeneous simple O-glycoproteomes (SimpleCell strategy), which enabled enrichment and sensitive mapping of the O-GalNAc and O-Man glycoproteomes of human cell lines. The development of isogenic cell lines differing in only one glycosyltransferase gene allows comparative studies to explore the function of a particular glycan or glycosylation pathway. This strategy was used to show that truncation of O-GalNAc glycans by targeting of the COSMC chaperone (<a href="/books/n/glyco3/ch10/?report=reader">Chapter 10</a>) induced oncogenic features (proliferation, growth, and invasive behavior) of human nontransformed keratinocytes, an interesting finding in light of the frequent overexpression of truncated O-glycans (Tn, STn) in cancer.</p><p>A related approach is to use glycoengineering for discovery of host glycans required for microbial and viral infectivity. In one remarkable study using binding of Lassa virus to a haploid cell line, the large number of the glycogenes required for synthesis of the extended O-Man glycans that support Lassa virus binding were identified and validated using a combination of selection for virus resistance and TALEN-mediated gene knockout.</p></div><div id="Ch56_s10"><h2 id="_Ch56_s10_">FUTURE PERSPECTIVES</h2><p>Glycoengineering of cells is entering a phase that may be described as “LEGO toying” due to the efficiency of precise gene editing. Entire glycosylation machineries can be deconstructed and rebuilt in various cell types. Cells show remarkable plasticity for engineering glycosylation pathways, with only a few glycosylation enzymes essential for cell growth in vitro. The essential functions for viability of mammalian cells are initial N-glycosylation (<a href="/books/n/glyco3/ch9/?report=reader">Chapter 9</a>) and nuclear/cytosolic O-GlcNAc modifications (<a href="/books/n/glyco3/ch19/?report=reader">Chapter 19</a>). These aside, we can envision that all glycosylation pathways in cells will be genetically deconstructed, and the roles of the genes determined. Combining engineering of glycosylation pathways in creative ways by introducing completely foreign enzymes can be used to produce novel glycans for study.</p><p>Large-scale glycosylation screening and discovery strategies are also possible. The CRISPR/Cas9 editing tool is particularly suited for multiplexed screening strategies, and whole-genome lentiviral-based knockout libraries have already been applied for screening mutations that result in altered biological function. Although knockdown strategies have been successful for screening biological functions of glycogenes in multiple organisms (worms, flies, frogs, and zebrafish), these have generally not been effective in mammalian cells due to low efficiency of knockdown. It is now possible to apply whole-glycogenome screening strategies in cell lines to probe and dissect the roles of glycosylation. These tools will dramatically improve the options for dissection of structure–function relationships in the field. The power of genetic deconvolution of an entire glycosylation pathway required for a biological function with a knockout screening strategy has already been shown with the Lassa virus study described above.</p><p>Glycoengineered cell lines and validated targeting constructs (knockout, knockin, and mutated) including libraries for screening will become important community resources that will advance the glycoscience field and help disseminate and integrate glycosciences more broadly in biology. It is possible to generate large libraries of cells with subtly different glycosylation. We can envision libraries with a combinatorial set of the 200+ identified mammalian glycosyltransferases that could serve as a platform for producing distinct glycoforms of any glycoconjugate, or as cell-based arrays displaying distinct glycoconjugates.</p><p>One word of caution should be raised: whereas glycoengineering by knockout is fairly straightforward, there is considerably more work needed to establish methods to build robust complex glycosylation capabilities requiring multiple gene insertions in cells. Nevertheless, we may envision large libraries of cells with different glycosylation capacities, including novel ones. Gene editing technologies have started a revolution in the glycoscience field, and we have only begun to see the new possibilities for manipulating glycosylation in cells and organisms, and exploiting glycoengineering in therapeutic glycoproteins and biologics</p></div><div id="ack53"><h2 id="_ack53_">ACKNOWLEDGMENTS</h2><p>The authors appreciate helpful comments and suggestions from Di Wu, Christopher Seaui, Benjamin Schulz, and Benjamin Schumann.</p></div><div id="rl56"><h2 id="_rl56_">FURTHER READING</h2><ul class="simple-list"><li class="half_rhythm"><p><div class="bk_ref" id="CH56C1">Wacker M, Linton D, Hitchen PG, Nita-Lazar M, Haslam SM, North SJ, Panico M, Morris HR, Dell A, Wren BW, et al.
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387–392. [<a href="https://pubmed.ncbi.nlm.nih.gov/17951046" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 17951046</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C3">Malphettes L, Freyvert Y, Chang J, Liu PQ, Chan E, Miller JC, Zhou Z, Nguyen T, Tsai C, Snowden AW, et al.
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2010. Highly efficient deletion of FUT8 in CHO cell lines using zinc-finger nucleases yields cells that produce completely nonfucosylated antibodies. Biotechnol Bioeng
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774–783. [<a href="https://pubmed.ncbi.nlm.nih.gov/20564614" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 20564614</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C4">North SJ, Huang HH, Sundaram S, Jang-Lee J, Etienne AT, Trollope A, Chalabi S, Dell A, Stanley P, Haslam SM. 2010. Glycomics profiling of Chinese hamster ovary cell glycosylation mutants reveals N-glycans of a novel size and complexity. J Biol Chem
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5759–5775. [<a href="/pmc/articles/PMC2820803/" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pmc">PMC free article<span class="bk_prnt">: PMC2820803</span></a>] [<a href="https://pubmed.ncbi.nlm.nih.gov/19951948" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 19951948</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C5">Baker JL, Celik E, DeLisa MP. 2013. Expanding the glycoengineering toolbox: the rise of bacterial N-linked protein glycosylation. Trends Biotechnol
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313–323. [<a href="https://pubmed.ncbi.nlm.nih.gov/23582719" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 23582719</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C6">Bosch D, Castilho A, Loos A, Schots A, Steinkellner H. 2013. N-glycosylation of plant-produced recombinant proteins. Curr Pharm Des
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5503–5512. [<a href="https://pubmed.ncbi.nlm.nih.gov/23394562" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 23394562</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C7">Merritt JH, Ollis AA, Fisher AC, DeLisa MP. 2013. Glycans-by-design: engineering bacteria for the biosynthesis of complex glycans and glycoconjugates. Biotechnol Bioeng
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1550–1564. [<a href="https://pubmed.ncbi.nlm.nih.gov/23456823" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 23456823</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C8">Steentoft C, Bennett EP, Schjoldager KT, Vakhrushev SY, Wandall HH, Clausen H. 2014. Precision genome editing: a small revolution for glycobiology. Glycobiology
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663–680. [<a href="https://pubmed.ncbi.nlm.nih.gov/24861053" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 24861053</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C9">Strasser R, Altmann F, Steinkellner H. 2014. Controlled glycosylation of plant-produced recombinant proteins. Curr Opin Biotechnol
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95–100. [<a href="https://pubmed.ncbi.nlm.nih.gov/25000187" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 25000187</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C10">Castilho A. 2015. Glyco-engineering. Preface. Methods Mol Biol
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1321:
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v–vii. [<a href="https://pubmed.ncbi.nlm.nih.gov/26280044" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 26280044</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C11">Laukens B, De Visscher C, Callewaert N. 2015. Engineering yeast for producing human glycoproteins: where are we now?
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Future Microbiol
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10:
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21–34. [<a href="https://pubmed.ncbi.nlm.nih.gov/25598335" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 25598335</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C12">Laukens B, De Wachter C, Callewaert N. 2015. Engineering the <em>Pichia pastoris</em> N-glycosylation pathway using the GlycoSwitch technology. Methods Mol Biol
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103–122. [<a href="https://pubmed.ncbi.nlm.nih.gov/26082218" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 26082218</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C13">Yang Z, Wang S, Halim A, Schulz MA, Frodin M, Rahman SH, Vester-Christensen MB, Behrens C, Kristensen C, Vakhrushev SY, et al.
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2015. Engineered CHO cells for production of diverse, homogeneous glycoproteins. Nat Biotechnol
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33:
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842–844. [<a href="https://pubmed.ncbi.nlm.nih.gov/26192319" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 26192319</span></a>]</div></p></li><li class="half_rhythm"><p><div class="bk_ref" id="CH56C14">Chiang AW, Li S, Spahn PN, Richelle A, Kuo CC, Samoudi M, Lewis NE. 2017. Modulating carbohydrate–protein interactions through glycoengineering of monoclonal antibodies to impact cancer physiology. Curr Opin Struct Biol
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40:
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104–111. [<a href="/pmc/articles/PMC5161599/" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pmc">PMC free article<span class="bk_prnt">: PMC5161599</span></a>] [<a href="https://pubmed.ncbi.nlm.nih.gov/27639240" ref="pagearea=cite-ref&targetsite=entrez&targetcat=link&targettype=pubmed">PubMed<span class="bk_prnt">: 27639240</span></a>]</div></p></li></ul></div><div id="bk_toc_contnr"></div></div></div><div class="fm-sec"><h2 id="_NBK453027_pubdet_">Publication Details</h2><h3>Author Information and Affiliations</h3><p class="contrib-group"><h4>Authors</h4><span itemprop="author">Henrik Clausen</span>, <span itemprop="author">Hans H. Wandall</span>, <span itemprop="author">Catharina Steentoft</span>, <span itemprop="author">Pamela Stanley</span>, and <span itemprop="author">Ronald L. Schnaar</span>.</p><h3>Publication History</h3><p class="small">Published online: 2017.</p><h3>Copyright</h3><div><div class="half_rhythm"><a href="/books/about/copyright/">Copyright</a> 2015-2017 by The Consortium of Glycobiology Editors, La Jolla, California. All rights reserved.<p class="small">PDF files are not available for download.</p></div></div><h3>Publisher</h3><p><a href="http://www.cshlpress.com/default.tpl?action=full&cart=12210755385880789&--eqskudatarq=666" ref="pagearea=page-banner&targetsite=external&targetcat=link&targettype=publisher">Cold Spring Harbor Laboratory Press</a>, Cold Spring Harbor (NY)</p><h3>NLM Citation</h3><p>Clausen H, Wandall HH, Steentoft C, et al. Glycosylation Engineering. 2017. In: Varki A, Cummings RD, Esko JD, et al., editors. Essentials of Glycobiology [Internet]. 3rd edition. Cold Spring Harbor (NY): Cold Spring Harbor Laboratory Press; 2015-2017. Chapter 56.<span class="bk_cite_avail"></span> doi: 10.1101/glycobiology.3e.056</p></div><div class="small-screen-prev"><a href="/books/n/glyco3/ch55/?report=reader"><svg xmlns="http://www.w3.org/2000/svg" viewBox="0 0 100 100" preserveAspectRatio="none"><path d="M75,30 c-80,60 -80,0 0,60 c-30,-60 -30,0 0,-60"></path><text x="20" y="28" textLength="60" style="font-size:25px">Prev</text></svg></a></div><div class="small-screen-next"><a href="/books/n/glyco3/ch57/?report=reader"><svg xmlns="http://www.w3.org/2000/svg" viewBox="0 0 100 100" preserveAspectRatio="none"><path d="M25,30c80,60 80,0 0,60 c30,-60 30,0 0,-60"></path><text x="20" y="28" textLength="60" style="font-size:25px">Next</text></svg></a></div></article><article data-type="fig" id="figobch56f1"><div id="ch56.f1" class="figure bk_fig"><div class="graphic"><img data-src="/books/NBK453027/bin/ch56f01.jpg" alt="FIGURE 56.1.. Overview of species-specific glycosylation features." /></div><h3><span class="label">FIGURE 56.1.</span></h3><div class="caption"><p>Overview of species-specific glycosylation features. The figure presents the different classes of glycoconjugates present in mammalian, plant, insect, and yeast cells with a representative glycan from each class. Structures to the right of the break are found in the cytoplasm and nucleus of the indicated organisms.</p></div><p><a href="/books/NBK453027/bin/ch56f01.pptx">Download Teaching Slide</a><span class="small"> (PPTX, 1.8M)</span></p></div></article><article data-type="table-wrap" id="figobCH56TB1"><div id="CH56TB1" class="table"><h3><span class="label">TABLE 56.1.</span></h3><div class="caption"><p>Examples of major achievements in glycoengineering of cells</p></div><p class="large-table-link" style="display:none"><span class="right"><a href="/books/NBK453027/table/CH56TB1/?report=objectonly" target="object">View in own window</a></span></p><div class="large_tbl" id="__CH56TB1_lrgtbl__"><table class="no_bottom_margin"><colgroup xmlns:mml="http://www.w3.org/1998/Math/MathML" xmlns:ali="http://www.niso.org/schemas/ali/1.0/" xmlns:xi="http://www.w3.org/2001/XInclude" xmlns:xsi="http://www.w3.org/2001/XMLSchema-instance" xmlns:pmc="http://www.pubmedcentral.gov/pmc" xmlns:xlink="http://www.w3.org/1999/xlink" span="1"><col align="left" span="1" /><col align="left" span="1" /><col align="left" span="1" /><col align="left" span="1" /><col align="left" span="1" /></colgroup><thead><tr><th id="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="text-align:left;vertical-align:top;">Cell</th><th id="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="text-align:left;vertical-align:top;">Gene modification</th><th id="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="text-align:left;vertical-align:top;">Effect</th><th id="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="text-align:left;vertical-align:top;">Purpose</th><th id="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="text-align:left;vertical-align:top;">Structure</th></tr></thead><tbody><tr><td headers="hd_h_CH56TB1_1_1_1_1 hd_h_CH56TB1_1_1_1_2 hd_h_CH56TB1_1_1_1_3 hd_h_CH56TB1_1_1_1_4 hd_h_CH56TB1_1_1_1_5" colspan="5" rowspan="1" style="vertical-align:top;">
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<b>Mammalian</b>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="vertical-align:top;">CHO</td><td headers="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="vertical-align:top;">KO of <i>Fut8</i></td><td headers="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="vertical-align:top;">elimination of core fucose</td><td headers="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="vertical-align:top;">IgG1 with increased ADCC</td><td headers="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="vertical-align:top;">
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<span class="graphic"><img src="/books/NBK453027/bin/ch56t01a.jpg" alt="Image ch56t01a.jpg" /></span>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="vertical-align:top;">CHO</td><td headers="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="vertical-align:top;">OE of <i>Mgat3</i></td><td headers="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="vertical-align:top;">reduction of core fucose by induction of bisecting GlcNAc</td><td headers="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="vertical-align:top;">IgG1 with increased ADCC</td><td headers="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="vertical-align:top;">
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<span class="graphic"><img src="/books/NBK453027/bin/ch56t01b.jpg" alt="Image ch56t01b.jpg" /></span>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="vertical-align:top;">CHO</td><td headers="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="vertical-align:top;">KO of 19 GTs combinations KI <i>ST6GalT1</i></td><td headers="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="vertical-align:top;">N-glycan deconstruction and reconstruction controlling branching, polyLacNAc, and sialylation</td><td headers="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="vertical-align:top;">design matrix to create homogeneous N-glycans of choice</td><td headers="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="vertical-align:top;">
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<span class="graphic"><img src="/books/NBK453027/bin/ch56t01c.jpg" alt="Image ch56t01c.jpg" /></span>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="vertical-align:top;">HEK293</td><td headers="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="vertical-align:top;">KO of <i>Mgat1</i> combined with Golgi-targeted expression of endo-β-N- acetylglucosaminidases</td><td headers="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="vertical-align:top;">single GlcNAc N-glycan “stumps” that can be recognized and modified by galactosyltransferases and sialyltransferases</td><td headers="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="vertical-align:top;">simple and homogenous N-glycosylation</td><td headers="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="vertical-align:top;">
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<span class="graphic"><img src="/books/NBK453027/bin/ch56t01d.jpg" alt="Image ch56t01d.jpg" /></span>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1 hd_h_CH56TB1_1_1_1_2 hd_h_CH56TB1_1_1_1_3 hd_h_CH56TB1_1_1_1_4 hd_h_CH56TB1_1_1_1_5" colspan="5" rowspan="1" style="vertical-align:top;">
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<b>Insect</b>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="vertical-align:top;">S2 <i>Drosophila melanogaster</i> cells</td><td headers="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="vertical-align:top;">introduction of sialic acid synthase, CMP-sialic acid synthase, CMP-sialic acid transporter, and a N-acetylglucosamine- 6- phosphate 2′-epimerase</td><td headers="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="vertical-align:top;">biantennary N-glycans with galactosylation and sialic acid</td><td headers="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="vertical-align:top;">human-like N-glycans in insect cells</td><td headers="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="vertical-align:top;">
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<span class="graphic"><img src="/books/NBK453027/bin/ch56t01e.jpg" alt="Image ch56t01e.jpg" /></span>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1 hd_h_CH56TB1_1_1_1_2 hd_h_CH56TB1_1_1_1_3 hd_h_CH56TB1_1_1_1_4 hd_h_CH56TB1_1_1_1_5" colspan="5" rowspan="1" style="vertical-align:top;">
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<b>Yeast</b>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="vertical-align:top;">
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<i>Yarrowia lipolytica</i>
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</td><td headers="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="vertical-align:top;">KO of <i>och</i><br />KI of <i>mnn4</i></td><td headers="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="vertical-align:top;">N-linked glycans with mannose-6-phosphates; uncapping can be performed in vitro with glycosidases and α-mannosidases</td><td headers="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="vertical-align:top;">lysosomal targeting of enzymes used for enzyme replacement in lysosomal storage diseases</td><td headers="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="vertical-align:top;">
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<span class="graphic"><img src="/books/NBK453027/bin/ch56t01f.jpg" alt="Image ch56t01f.jpg" /></span>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="vertical-align:top;">
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<i>Pichia pastorius</i>
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</td><td headers="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="vertical-align:top;">KO of <i>ochl</i>, <i>pnol</i>, <i>mnn4B</i>, <i>bmt2</i>; KI of 14 genes: UDP-GlcNAc transporters, MnsI, <i>Mgat1</i>, <i>Mgat2</i>, <i>MnsII</i>, Gal epimerase, UDP-Gal transporter, B4GalT1, and sialic acid biosynthetic pathway, and transporters</td><td headers="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="vertical-align:top;">biantennary N-linked glycans with sialylation</td><td headers="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="vertical-align:top;">human-like N-glycans in yeast</td><td headers="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="vertical-align:top;">
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<span class="graphic"><img src="/books/NBK453027/bin/ch56t01g.jpg" alt="Image ch56t01g.jpg" /></span>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="vertical-align:top;">
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<i>P. pastorius</i>
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</td><td headers="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="vertical-align:top;">KO of <i>ochl</i>; OE of <i>Mgat1</i>, <i>B4galt1</i> targeted to Golgi and α2-mannosidase retained in the endoplasmic reticulum</td><td headers="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="vertical-align:top;">biantennary N-linked glycans with either 2, 3 or 2, 6 sialylation</td><td headers="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="vertical-align:top;">human-like N-glycan core in yeast</td><td headers="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="vertical-align:top;">
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<span class="graphic"><img src="/books/NBK453027/bin/ch56t01h.jpg" alt="Image ch56t01h.jpg" /></span>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1 hd_h_CH56TB1_1_1_1_2 hd_h_CH56TB1_1_1_1_3 hd_h_CH56TB1_1_1_1_4 hd_h_CH56TB1_1_1_1_5" colspan="5" rowspan="1" style="vertical-align:top;">
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<b>Bacteria</b>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="vertical-align:top;">
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<i>Escherichia coli</i>
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</td><td headers="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="vertical-align:top;">introducing OST PglB from <i>Campylobacter jejuni</i> together with four glyco-syltransferases from <i>Saccharomyces cerevisiae</i> encoded by KI, <i>ALG1</i>, <i>ALG2</i>, <i>ALG13</i>, and <i>ALG14</i></td><td headers="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="vertical-align:top;">introduce N-glycosylation into major prokaryotic production organism</td><td headers="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="vertical-align:top;">mammalian core Man3GlcNAc2 glycostructure</td><td headers="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="vertical-align:top;">
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<span class="graphic"><img src="/books/NBK453027/bin/ch56t01i.jpg" alt="Image ch56t01i.jpg" /></span>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1 hd_h_CH56TB1_1_1_1_2 hd_h_CH56TB1_1_1_1_3 hd_h_CH56TB1_1_1_1_4 hd_h_CH56TB1_1_1_1_5" colspan="5" rowspan="1" style="vertical-align:top;">
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<b>Plants</b>
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</td></tr><tr><td headers="hd_h_CH56TB1_1_1_1_1" rowspan="1" colspan="1" style="vertical-align:top;">
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<i>Nicotiana tabacum</i>
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</td><td headers="hd_h_CH56TB1_1_1_1_2" rowspan="1" colspan="1" style="vertical-align:top;">KO of β-hexosaminidase, α3-fucosyltransferase, and β2-xylosyltransferase; KI of <i>B4galt1</i>, ST6GalI, and CMP-NeuAc synthase and transporters</td><td headers="hd_h_CH56TB1_1_1_1_3" rowspan="1" colspan="1" style="vertical-align:top;">production of biantennary N-glycans without core fucose and α2-6NeuAc</td><td headers="hd_h_CH56TB1_1_1_1_4" rowspan="1" colspan="1" style="vertical-align:top;">human-like N-glycans in plants</td><td headers="hd_h_CH56TB1_1_1_1_5" rowspan="1" colspan="1" style="vertical-align:top;">
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<span class="graphic"><img src="/books/NBK453027/bin/ch56t01j.jpg" alt="Image ch56t01j.jpg" /></span>
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</td></tr></tbody></table></div><div class="tblwrap-foot"><div><dl class="temp-labeled-list small"><dl class="bkr_refwrap"><dt></dt><dd><div><p class="no_margin">CHO, Chinese hamster ovary; KO, knockout; OE, overexpress; KI, knockin; CMP, cytidine monophosphate; OST, oligosaccharyltransferase; ADCC, antigen-dependent cellular cytotoxicity.</p></div></dd></dl></dl></div></div></div></article><article data-type="fig" id="figobch56f2"><div id="ch56.f2" class="figure bk_fig"><div class="graphic"><img data-src="/books/NBK453027/bin/ch56f02.jpg" alt="FIGURE 56.2.. Precise gene editing modalities." /></div><h3><span class="label">FIGURE 56.2.</span></h3><div class="caption"><p>Precise gene editing modalities. Glycosyltransferases are represented with their catalytic domains and amino-terminal membrane spanning domains. Examples of gene edition for gene disruption (knockout), editing (mutation), tagging, and insertion of heterologous glycosyltransferases at a “safe harbor” locus are shown. Precise gene editing uses targeted nucleases to introduce double-stranded DNA breaks at specific locations. In mammalian cells, these breaks are repaired by nonhomologous end joining (NHEJ) or homologous recombination (HR). NHEJ is an error-prone mechanism that often introduces small insertions or deletions (Indels) resulting in frameshift mutations. Editing (to introduce targeted mutations) or insertion of glycosyltransferase genes mainly relies on HR following cotransfection of appropriate donor DNA constructs. For efficient knockout of type 2 transmembrane glycosyltransferases, it is often sufficient to target one of the first coding exons, which leads to nonsense-mediated decay of mRNA or causes alternative splicing that usually gives rise to nonfunctional proteins, but more generally it is advisable to target functional domains.</p></div><p><a href="/books/NBK453027/bin/ch56f02.pptx">Download Teaching Slide</a><span class="small"> (PPTX, 1.8M)</span></p></div></article><article data-type="fig" id="figobch56f3"><div id="ch56.f3" class="figure bk_fig"><div class="graphic"><img data-src="/books/NBK453027/bin/ch56f03.jpg" alt="FIGURE 56.3.. Complex N-glycan with glycosyltransferases responsible for each reaction." /></div><h3><span class="label">FIGURE 56.3.</span></h3><div class="caption"><p>Complex N-glycan with glycosyltransferases responsible for each reaction. Combinatorial knockout of the glycosyltransferase isoenzyme genes indicated led to the identification of the primary genes (highlighted in bold) controlling N-glycan branching (MGATs), elongation (β3GlcNAc-Ts and β4Gal-Ts), and sialylation (ST3GALs) in CHO cells.</p></div><p><a href="/books/NBK453027/bin/ch56f03.pptx">Download Teaching Slide</a><span class="small"> (PPTX, 1.7M)</span></p></div></article></div><div id="jr-scripts"><script src="/corehtml/pmc/jatsreader/ptpmc_3.22/js/libs.min.js"> </script><script src="/corehtml/pmc/jatsreader/ptpmc_3.22/js/jr.min.js"> </script></div></div>
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