
{"id":16876,"date":"2026-03-16T14:04:13","date_gmt":"2026-03-16T14:04:13","guid":{"rendered":"https:\/\/www.sygnaturediscovery.com\/blog\/welcoming-expicho-s-to-our-mammalian-expression-portfolio\/"},"modified":"2026-03-16T14:04:13","modified_gmt":"2026-03-16T14:04:13","slug":"welcoming-expicho-s-to-our-mammalian-expression-portfolio","status":"publish","type":"blog","link":"https:\/\/www.sygnaturediscovery.com\/fr\/blog\/welcoming-expicho-s-to-our-mammalian-expression-portfolio\/","title":{"rendered":"Welcoming ExpiCHO-S to our mammalian expression portfolio"},"content":{"rendered":"\n<h2 class=\"wp-block-heading has-dark-blue-500-color has-text-color has-link-color has-text-2-xl-font-size wp-elements-e568f48ef1d4bc666f4f700708a31b56\">The <a href=\"https:\/\/www.sygnaturediscovery.com\/fr\/solutions-scientifiques\/science-des-proteines-et-biologie-structurale\/\" target=\"_blank\" rel=\"noreferrer noopener\">Protein &amp; Structure department<\/a> at Sygnature Discovery are excited to announce <strong>ExpiCHO\u2011S<sup>TM<\/sup><\/strong> as the latest addition to our mammalian expression platform. This expansion of cell line capabilities further enhances the flexibility and scalability of the recombinant protein expression services we provide to clients across biotech and pharma.<\/h2>\n\n\n\n<p>As part of the onboarding process, we compared expression of various test proteins, including 4 antibodies in <strong>ExpiCHO\u2011S<sup>TM<\/sup><\/strong> with our well-established CHO-3E7 cell line and we present that data below.<\/p>\n\n\n\n<h2 class=\"wp-block-heading has-dark-blue-500-color has-text-color has-link-color has-text-2-xl-font-size wp-elements-9735fab11a6638d10ed1a2f91c5a41bf\">Choosing the Right Cell Line Matters<\/h2>\n\n\n\n<p>It has always been our philosophy to choose the expression host cell based on the nature of protein target itself and where there are multiple possible options, to perform a comparison screen early in a programme. Different targets respond differently to each system, and selecting the right platform from the outset can:<\/p>\n\n\n\n<ul class=\"wp-block-list\">\n<li>improve yields<\/li>\n\n\n\n<li>reduce development timelines<\/li>\n\n\n\n<li>minimise costs<\/li>\n\n\n\n<li>ensure delivery of the required protein quantity and quality<\/li>\n<\/ul>\n\n\n\n<p>Within our Cell Science team, we offer a diverse suite of eukaryotic expression systems to support proteins of varying complexity and production needs. Our portfolio now includes:<\/p>\n\n\n\n<ul class=\"wp-block-list\">\n<li>HEK293\u20116E and CHO\u20113E7 (both licensed from the National Research Council, Canada)<\/li>\n\n\n\n<li>Expi293\u2122 and ExpiCHO\u2011S<sup>TM<\/sup> (both licensed from Thermo Fisher Scientific)<\/li>\n<\/ul>\n\n\n\n<h2 class=\"wp-block-heading has-dark-blue-500-color has-text-color has-link-color has-text-2-xl-font-size wp-elements-5d5dda4b4c1303cdad3cfecbd01aa62a\">Why do we need mammalian expression platforms?<\/h2>\n\n\n\n<p>Mammalian expression platforms are essential for producing proteins that closely replicate their natural human counterparts, making them vital for both research and biotherapeutic development. Unlike bacterial or insect systems, mammalian cells provide the full repertoire of human\u2011like post\u2011translational modifications (PTMs)\u2014particularly glycosylation, disulfide bond formation, and complex folding pathways\u2014that many secreted, membrane, and multi\u2011subunit proteins require to be stable and functional. These systems also offer the appropriate lipid environment, chaperones, and trafficking machinery needed for challenging targets such as GPCRs, cytokines, and antibodies. As a result, mammalian platforms such as CHO and HEK293 have become the industry standard for generating biologically relevant and regulatory\u2011compliant protein material, underpinning the production of most approved therapeutics and enabling high\u2011fidelity studies of protein structure and function.<\/p>\n\n\n\n<h2 class=\"wp-block-heading has-dark-blue-500-color has-text-color has-link-color has-text-2-xl-font-size wp-elements-c6cc02519bc1ea5739accc81dbed6eb8\">Comparing ExpiCHO-S<sup>TM<\/sup> to CHO-3E7<\/h2>\n\n\n\n<p>With an increasing demand for high\u2011yield mammalian expression systems, we evaluated ExpiCHO\u2011S<sup>TM<\/sup> to understand where it fits relative to our existing mammalian platforms.<\/p>\n\n\n\n<p>For this comparison we selected a range of test proteins<\/p>\n\n\n\n<ul class=\"wp-block-list\">\n<li>TIMP2 is a well\u2011characterised secreted protein, which we have produced extensively across several cell lines. TIMP2 exhibits intermediate expression levels, making it an excellent benchmark for detecting improvements or shifts in productivity between systems.<\/li>\n\n\n\n<li>Two mCherry tagged proteins, one intracellular and the other that is secreted<\/li>\n\n\n\n<li>Four recombinant antibodies: Depemokimab, Bococizumab, Eldelumab, and Sacituzumab<\/li>\n<\/ul>\n\n\n\n<p>For each of these proteins we compared:<\/p>\n\n\n\n<ul class=\"wp-block-list\">\n<li>CHO\u20113E7, as a control using our internally optimised expression workflow<\/li>\n\n\n\n<li>ExpiCHO\u2011S<sup>TM<\/sup>, using the Thermo Fisher ExpiCHO\u2122 Expression System Kit<\/li>\n<\/ul>\n\n\n\n<h3 class=\"wp-block-heading has-blue-400-color has-text-color has-link-color has-text-xl-font-size wp-elements-432700d44d68b1384760b982b7c027f4\">Overview of the ExpiCHO-S<sup>TM <\/sup>protocols<\/h3>\n\n\n\n<p>Alongside the cells Thermo Fisher also provides three recommended expression protocols for ExpiCHO\u2011S<sup>TM<\/sup>\u2014called STANDARD, HIGH, and MAX\u2014each incorporating different feeding and temperature\u2011shift strategies to enhance protein yield.<\/p>\n\n\n\n<p><strong>STANDARD protocol:<\/strong><\/p>\n\n\n\n<ul class=\"wp-block-list\">\n<li>Transfection at 37\u00b0C<\/li>\n\n\n\n<li>Addition of enhancer and feed at 24 h post\u2011transfection<\/li>\n\n\n\n<li>Culture maintained at 37\u00b0C to harvest (Day 8-10)<\/li>\n<\/ul>\n\n\n\n<p><strong>HIGH protocol:<\/strong><\/p>\n\n\n\n<ul class=\"wp-block-list\">\n<li>Same transfection\/enhancer\/feed schedule as STANDARD protocol<\/li>\n\n\n\n<li>Temperature shift to 32\u00b0C after the 24 h feed<\/li>\n\n\n\n<li>Culture maintained at 32\u00b0C to harvest (Day 10-12)<\/li>\n<\/ul>\n\n\n\n<p><strong>MAX protocol:<\/strong><\/p>\n\n\n\n<ul class=\"wp-block-list\">\n<li>Same transfection\/enhancer\/feed schedule as STANDARD\/HIGH protocol<\/li>\n\n\n\n<li>Temperature shift to 32\u00b0C after the 24 h feed<\/li>\n\n\n\n<li>Second feed (day 5)<\/li>\n\n\n\n<li>Culture maintained at 32\u00b0C to harvest (Day 12-14)<\/li>\n\n\n\n<li>Designed to maximise productivity<\/li>\n<\/ul>\n\n\n\n<figure class=\"wp-block-image size-full is-style-rounded is-style-rounded--1\"><img loading=\"lazy\" decoding=\"async\" width=\"963\" height=\"539\" src=\"https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/ExpiCHO-Protocol-Comparison.webp\" alt=\"\" class=\"wp-image-16485\" srcset=\"https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/ExpiCHO-Protocol-Comparison.webp 963w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/ExpiCHO-Protocol-Comparison-300x168.webp 300w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/ExpiCHO-Protocol-Comparison-768x430.webp 768w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/ExpiCHO-Protocol-Comparison-640x358.webp 640w\" sizes=\"(max-width: 963px) 100vw, 963px\"><figcaption class=\"wp-element-caption\">Figure 1: Schematic of ExpiCHO and CHO-3E7 transfection protocols. <\/figcaption><\/figure>\n\n\n\n<p><\/p>\n\n\n\n<h3 class=\"wp-block-heading has-blue-400-color has-text-color has-link-color has-text-xl-font-size wp-elements-a618d6cbffcc7338155eddda20002a86\">TIMP2: Greater yields observed across all ExpiCHO-S<sup>TM <\/sup>protocols<\/h3>\n\n\n\n<p>Our evaluation of secreted TIMP2 demonstrated a marked improvement in expression across all three supplied ExpiCHO\u2011S<sup>TM<\/sup> protocols (Figure\u202f2, left). Each expression workflow\u2014STANDARD, HIGH and MAX\u2014produced substantially higher titres than our established CHO\u20113E7 process for this particular protein, highlighting the robustness of the ExpiCHO\u2011S<sup>TM<\/sup> system even without any additional optimisation.<\/p>\n\n\n\n<figure class=\"wp-block-image size-full is-style-rounded is-style-rounded--2\"><img loading=\"lazy\" decoding=\"async\" width=\"945\" height=\"522\" src=\"https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/TIMP2-Expression-in-CHO-Comparison.webp\" alt=\"\" class=\"wp-image-16484\" srcset=\"https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/TIMP2-Expression-in-CHO-Comparison.webp 945w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/TIMP2-Expression-in-CHO-Comparison-300x166.webp 300w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/TIMP2-Expression-in-CHO-Comparison-768x424.webp 768w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/TIMP2-Expression-in-CHO-Comparison-640x354.webp 640w\" sizes=\"(max-width: 945px) 100vw, 945px\"><figcaption class=\"wp-element-caption\">Figure 2. Coomassie stain (left) and Anti-His HRP-mouse monoclonal, chemiluminescence (right) after Day 8 harvest in both CHO-3E7 and ExpiCHO-STM. <\/figcaption><\/figure>\n\n\n\n<h3 class=\"wp-block-heading has-blue-400-color has-text-color has-link-color has-text-xl-font-size wp-elements-4ed90be18c6fd60e2a0f6660b8011a3d\">mCherry secreted construct<\/h3>\n\n\n\n<p>The trend seen with TIMP2 was further supported by our secreted mCherry control construct (Figure\u202f3, right). The parallel increase in expression for both TIMP2 and mCherry indicates that the observed improvements are system\u2011driven rather than target\u2011specific.<\/p>\n\n\n\n<p>Together with the TIMP2 data, these results strongly suggest that ExpiCHO\u2011S<sup>TM<\/sup>, used in combination with the supplied manufacturer\u2011recommended protocols, represents an excellent addition to our mammalian expression portfolio for secreted proteins and provides clients with a high\u2011yield alternative to our existing CHO platform.<\/p>\n\n\n\n<h3 class=\"wp-block-heading has-blue-400-color has-text-color has-link-color has-text-xl-font-size wp-elements-a54df83245591f7f3878f544a56524d2\">mCherry intracellular construct<\/h3>\n\n\n\n<p>Interestingly, the expression of an intracellular mCherry control construct did <em>not<\/em> show a comparable improvement in ExpiCHO\u2011S<sup>TM<\/sup> cells (Figure\u202f3, left). When benchmarked against our in\u2011house CHO\u20113E7 platform, intracellular mCherry levels remained broadly similar, suggesting no clear advantage to switching systems for cytosolic targets. Given the higher media and transfection reagent costs associated with ExpiCHO\u2011S<sup>TM<\/sup>, these findings indicate that CHO\u20113E7 may remain the more cost\u2011effective choice for intracellular protein production.<\/p>\n\n\n\n<figure class=\"wp-block-image size-large is-style-rounded is-style-rounded--3\"><img loading=\"lazy\" decoding=\"async\" width=\"1024\" height=\"462\" src=\"https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/mCherry-constructs-Expression-in-CHO-1024x462.webp\" alt=\"\" class=\"wp-image-16483\" srcset=\"https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/mCherry-constructs-Expression-in-CHO-1024x462.webp 1024w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/mCherry-constructs-Expression-in-CHO-300x135.webp 300w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/mCherry-constructs-Expression-in-CHO-768x346.webp 768w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/mCherry-constructs-Expression-in-CHO-640x289.webp 640w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/mCherry-constructs-Expression-in-CHO.webp 1169w\" sizes=\"(max-width: 1024px) 100vw, 1024px\"><figcaption class=\"wp-element-caption\">Figure 3. mCherry control expression from an intracellular (left) and secreted (right) control construct.<\/figcaption><\/figure>\n\n\n\n<p><\/p>\n\n\n\n<h3 class=\"wp-block-heading has-blue-400-color has-text-color has-link-color has-text-xl-font-size wp-elements-b74189690c4534f5a2dd37a2b75fa19a\">Recombinant Antibody Production: Strong Performance in ExpiCHO\u2011S<sup>TM<\/sup><\/h3>\n\n\n\n<p>Finally, we evaluated recombinant antibody expression in ExpiCHO\u2011S<strong><sup>TM<\/sup><\/strong> and found that <strong>this system can achieve yields approaching 1<\/strong><strong>\u202fg\/L<\/strong>, underscoring its suitability for demanding biotherapeutic projects.<\/p>\n\n\n\n<p>Using the Thermo MAX protocol (described above), we expressed His\u2011tagged Depemokimab and Eldelumab, followed by nickel\u2011affinity purification. Both antibodies showed substantially higher yields in ExpiCHO\u2011S<sup>TM<\/sup> relative to our in\u2011house CHO\u20113E7 platform\u2014a 6\u2011fold increase for Depemokimab and an 11\u2011fold increase for Eldelumab. In contrast, Bococizumab displayed only a modest improvement, with a 1.5\u2011fold increase in ExpiCHO\u2011S<sup>TM<\/sup> (Figure\u202f4, right), reinforcing that performance gains remain target\u2011specific.<\/p>\n\n\n\n<p>Building on this, we expressed Sacituzumab using the Thermo MAX protocol and purified it under low\u2011endotoxin conditions via Protein A affinity chromatography. The resulting high\u2011yield, clean preparation further strengthened our confidence in ExpiCHO\u2011S<sup>TM<\/sup> as a robust platform for recombinant antibody production (Figure 4, left).<\/p>\n\n\n\n<figure class=\"wp-block-image size-large is-style-rounded is-style-rounded--4\"><img loading=\"lazy\" decoding=\"async\" width=\"1024\" height=\"438\" src=\"https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/Comparison-of-4-antibodies-expression-in-CHO-1024x438.webp\" alt=\"\" class=\"wp-image-16482\" srcset=\"https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/Comparison-of-4-antibodies-expression-in-CHO-1024x438.webp 1024w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/Comparison-of-4-antibodies-expression-in-CHO-300x128.webp 300w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/Comparison-of-4-antibodies-expression-in-CHO-768x329.webp 768w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/Comparison-of-4-antibodies-expression-in-CHO-640x274.webp 640w, https:\/\/www.sygnaturediscovery.com\/wp-content\/uploads\/2026\/03\/Comparison-of-4-antibodies-expression-in-CHO.webp 1147w\" sizes=\"(max-width: 1024px) 100vw, 1024px\"><figcaption class=\"wp-element-caption\">Figure 4. Coomassie staining of Sacituzumab supernatant at day 8, 11 and 13 and Protein A affinity chromatography-purified fractions (left) and summary of recombinant antibody yields in ExpiCHO-STM and CHO-3E7 (right).<\/figcaption><\/figure>\n\n\n\n<p><\/p>\n\n\n\n<h2 class=\"wp-block-heading has-dark-blue-500-color has-text-color has-link-color has-text-2-xl-font-size wp-elements-dca1e3e8e7300c20111e77077e1a3f6f\">In Summary<\/h2>\n\n\n\n<p>Our evaluation has shown that the ExpiCHO\u2011S<strong><sup>TM<\/sup><\/strong> cell line can have clear advantages for high yielding expression of secreted protein targets, especially antibodies, and is a valuable addition to our mammalian host cell portfolio that we offer.<\/p>\n\n\n\n<p>At Sygnature Discovery, we work closely with clients to identify the most suitable expression strategy for each target and project, supporting efficient and scalable routes to recombinant protein production.<\/p>\n","protected":false},"excerpt":{"rendered":"","protected":false},"featured_media":16877,"template":"","category":[1407],"class_list":["post-16876","blog","type-blog","status-publish","has-post-thumbnail","hentry","category-protein-expression-and-purification"],"acf":[],"yoast_head":"<!-- This site is optimized with the Yoast SEO plugin v27.4 - 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