Stable antibody expression at therapeutic levels using the 2A peptide

Fang, Jianming; Qian, Jingjing; Yi, Saili; Harding, Thomas C.; Tu, Guang Huan; VanRoey, Melinda; Jooss, Karin

doi:10.1038/nbt1087

Cited by 348 publications

(383 citation statements)

References 33 publications

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“…All the constructs, irrelevant to the origin of 2A peptides (T2A, F2A, P2A), functioned to produce the TCR in these two cell lines as demonstrated by fluorescence-activated cell sorting (FACS) analysis following gp100 tetramer staining ( Figure 1c). In contrast to a previous report, 29 the addition of furin to the 2A peptide inhibited TCR expression, whereas furin plus the addition of spacer sequences (GSG or SGSG) enabled highly efficient gene expression (up to 95%). While active in T-cell lines, these constructs produced significantly less TCR in primary PBL (o34% tetramer+; Supplementary Figure 1).…”

Section: A Peptides Along With Furin and Spacer Facilitate Transgenecontrasting

confidence: 96%

Development of optimal bicistronic lentiviral vectors facilitates high-level TCR gene expression and robust tumor cell recognition

et al. 2008

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In human gene therapy applications, lentiviral vectors may have advantages over g-retroviral vectors in several areas, including the ability to transduce nondividing cells, resistance to gene silencing and a potentially safer integration site profile. However, unlike g-retroviral vectors it has been problematic to drive the expression of multiple genes efficiently and coordinately with approaches such as internal ribosome entry sites or dual promoters. Using different 2A peptides, lentiviral vectors expressing two-gene T-cell receptors directed against the melanoma differentiation antigens gp100 and MART-1 were constructed. We demonstrated that addition of amino-acid spacer sequences (GSG or SGSG) before the 2A sequence is a prerequisite for efficient synthesis of biologically active T-cell receptors and that addition of a furin cleavage site followed by a V5 peptide tag yielded optimal T-cell receptor gene expression. Furthermore, we determined that the furin cleavage site was recognized in lymphocytes and accounted for removal of residual 2A peptides at the post-translational level with an efficiency of 20-30%, which could not be increased by addition of multiple furin cleavage sites. The novel bicistronic lentiviral vector developed herein afforded robust antimelanoma activities to engineered peripheral blood lymphocytes, including cytokine secretion, cell proliferation and lytic activity. Such optimal vectors may have immediate applications in cancer gene therapy.

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Section: A Peptides Along With Furin and Spacer Facilitate Transgenecontrasting

confidence: 96%

Development of optimal bicistronic lentiviral vectors facilitates high-level TCR gene expression and robust tumor cell recognition

et al. 2008

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“…This result, together with Western blot analysis, confirmed that fully assembled bioactive antibody complex was successfully produced from the IntF2A‐based polyprotein system. With the N‐extein linker‐free IntF2A system, the processed antibody light chain preserved its authentic C‐terminus without addition of any residual amino acids, which is superior to previously reported approaches (Fang et al ., 2005). The native N‐terminus of the processed downstream heavy chain fragment should also be preserved as the proline residue introduced by the action of F2A is removed upon signal peptide cleavage.…”

Section: Resultsmentioning

confidence: 99%

Coordinated protein co‐expression in plants by harnessing the synergy between an intein and a viral 2A peptide

Zhang

Rapolu

Kumar³

et al. 2017

Plant Biotechnology Journal

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SummaryA novel approach is developed for coordinated expression of multiple proteins from a single transgene in plants. An Ssp DnaE mini‐intein variant engineered for hyper‐N‐terminal autocleavage is covalently linked to the foot‐and‐mouth disease virus 2A (F2A) peptide with unique ribosome skipping property, via a peptide linker, to create an ‘IntF2A’ self‐excising fusion protein domain. This IntF2A domain acts, in cis, to direct highly effective release of its flanking proteins of interest (POIs) from a ‘polyprotein’ precursor in plants. This is successfully demonstrated in stably transformed cultured tobacco cells as well as in different organs of transgenic tobacco plants. Highly efficient polyprotein processing mediated by the IntF2A domain was also demonstrated in lettuce and Nicotiana benthamiana based on transient expression. Protein constituents released from the polyprotein precursor displayed proper function and accumulated at similar levels inside the cells. Importantly, no C‐terminal F2A extension remains on the released POIs. We demonstrated co‐expression of as many as three proteins in plants without compromising expression levels when compared with those using single‐protein vectors. Accurate differential cellular targeting of released POIs is also achieved. In addition, we succeeded in expressing a fully assembled and functional chimeric anti‐His Tag antibody in N. benthamiana leaves. The IntF2A‐based polyprotein transgene system overcomes key impediments of existing strategies for multiprotein co‐expression in plants, which is particularly important for gene/trait stacking.

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“…To produce a stoichiometric amount of the heavy and light antibody chain, the effector construct was designed as a single mRNA transcript comprising coding sequences for three polypeptide chains, an anti-hTNF-a antibody heavy chain, an anti-hTNF-a antibody light chain, and hIL-1RA or mIL-10. The polypeptide-coding chains were linked through the coding sequence for the 2A peptide, which interrupts the translation of the polypeptide chain, similar as described previously 34 ( Figure 5A). These composite anti-inflammatory therapeutics were integrated in the final effector constructs pAS116 (TRE-UAS-P MIN -anti-hTNF-a Ab-hIL-1RA) and pAS134 (TRE-UAS-P MIN -anti-hTNF-a Ab-mIL-10, Table S1).…”

Section: Design and Biological Activity Of The Composite Antiinflammamentioning

confidence: 99%

A Synthetic Mammalian Therapeutic Gene Circuit for Sensing and Suppressing Inflammation

et al. 2017

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Stable antibody expression at therapeutic levels using the 2A peptide

Cited by 348 publications

References 33 publications

Development of optimal bicistronic lentiviral vectors facilitates high-level TCR gene expression and robust tumor cell recognition

Development of optimal bicistronic lentiviral vectors facilitates high-level TCR gene expression and robust tumor cell recognition

Coordinated protein co‐expression in plants by harnessing the synergy between an intein and a viral 2A peptide

A Synthetic Mammalian Therapeutic Gene Circuit for Sensing and Suppressing Inflammation

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