2020
DOI: 10.1080/19420862.2020.1829334
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Functional humanization of immunoglobulin heavy constant gamma 1 Fc domain human FCGRT transgenic mice

Abstract: A major asset of many monoclonal antibody (mAb)-based biologics is their persistence in circulation. The MHC class I family Fc receptor, FCGRT, is primarily responsible for this extended pharmacokinetic behavior. Engagement of FCGRT with the crystallizable fragment (Fc) domain protects IgG from catabolic elimination, thereby extending the persistence and bioavailability of IgG and related Fc-based biologics. There is a need for reliable in vivo models to facilitate the preclinical development of novel IgG-base… Show more

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Cited by 11 publications
(15 citation statements)
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“…Of note is that the β phase t ½ for i.v. trastuzumab, currently in human use, is ∼8.5 days in Tg32 mice (31)––this latter β decay translates into 21–day dosing intervals.…”
Section: Resultsmentioning
confidence: 99%
“…Of note is that the β phase t ½ for i.v. trastuzumab, currently in human use, is ∼8.5 days in Tg32 mice (31)––this latter β decay translates into 21–day dosing intervals.…”
Section: Resultsmentioning
confidence: 99%
“…Interestingly, a modified version of the Tg32 strain has been recently reported to produce hIgG1 Fc combined with mIgG Fab arms, which is rescued by hFcRn (Fig. 5B) [219]. The levels of endogenous chimeric mouse-human IgG1 were shown to be greatly increased upon immunization, which modulated the half-life of injected hIgG.…”
Section: Human Fcrn Transgenic Mouse Modelsmentioning
confidence: 91%
“…To solve this preclinical challenge, several genetically engineered mouse strains have been developed where the mFcRn heavy chain has been replaced with the human counterpart, either under the control of mouse or human promoter elements [32,74,181,216,[219][220][221][222][223]. These strains are the current gold standards for the evaluation of hFcRn-targeting strategies addressing pharmacokinetics, pharmacodynamics and delivery across selective mucosal barriers prior to studies in non-human primates.…”
Section: Human Fcrn Transgenic Mouse Modelsmentioning
confidence: 99%
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“…CRISPR-driven humanization of large regions of the mouse genome represents a challenging process that, in addition to CAS9 and gRNA, requires the co-injection of repair template DNA, designed to trigger the cells' homology-directed repair pathway, into the nucleus of a 1-cell mouse zygote. Whilst this approach has been successfully used to humanize gene coding regions in mice [62][63][64], it has yet to be used to humanize enhancer regions. The alternative, and more conventional, strategy to humanization involves embryonic stem (ES)-cell targeting and blastocyst microinjection [65].…”
Section: Conserved Enhancers In Adult Brain Activitymentioning
confidence: 99%