Rapid and reliable cloning of antibody variable regions and generation of recombinant single chain antibody fragments

分子生物学 生物 基因 互补DNA 底漆(化妆品) 重组DNA 抗体 病毒学 遗传学 化学 有机化学
作者
Lisa K. Gilliland,Nancy Norris,Hans Marquardt,T T Tsu,Martha S. Hayden,Michael Neubauer,D E Yelton,Robert S. Mittler,J A Ledbetter
出处
期刊:Tissue Antigens [Wiley]
卷期号:47 (1): 1-20 被引量:57
标识
DOI:10.1111/j.1399-0039.1996.tb02509.x
摘要

Abstract: Single chain antibody variable region fragments (sFv), by virtue of their size and method of construction are potentially useful as therapeutic reagents and as tools for exploring cell surface receptor function. sFv offer several advantages over the intact immunoglobulin molecule. For instance, they are expressed from a single transcript and can be molecularly linked to other proteins to generate bispecific sFv molecules or single‐chain immunotoxins. The relatively small size of sFv is an advantage in allowing for easier penetrance into tissue spaces, and their clearance rate is exceedingly rapid. sFv are useful for gene therapy since they can be directed to a specific cellular localization and can be fused to retroviral env genes to control viral host range. To prepare sFv to murine and human leukocyte CD antigens, we devised a method for rapid cloning and expression that can yield functional protein within 2–3 weeks of RNA isolation from hybridoma cells. The variable regions were cloned by poly‐G tailing the first strand cDNA followed by anchor PCR with a forward poly‐C anchor primer and a reverse primer specific for constant region sequence. Both primers contain flanking restriction sites for insertion into PUC19. Sets of PCR primers for isolation of murine, hamster and rat VL and VH genes were generated. Following determination of consensus sequences for a specific VL and VH pair, the VL and VH genes were linked by DNA encoding an intervening peptide linker [usually (Gly4Ser)3] and the VL‐link‐VH gene cassettes were transferred into the pCDM8 mammalian expression vector. The constructs were transfected into COS cells and sFvs were recovered from spent culture supernatant. We have used this method to generate functional sFv to human CD2, CD3, CD4, CD8, CD28, CD40, CD45 and to murine CD3 and gp39, from hybridomas producing murine, rat, or hamster antibodies. Initially, the sFvs were expressed as fusion proteins with the hinge‐CH2‐CH3 domains of human IgG1 to facilitate rapid characterization and purification using goat anti‐human IgG reagents or protein A. We also found that active sFv could be expressed with a small peptide <tag< or in a tail‐less form. Expression of CD3 (G19–4) sFv tail‐less or Ig tailed forms demonstrated increased cellular signalling activity and suggested that sFv have potential for activating receptors.
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