首页> 外文期刊>Protein Engineering >SINGLE-CHAIN FV FRAGMENTS OF ANTI-NEURAMINIDASE ANTIBODY NC10 CONTAINING FIVE- AND TEN-RESIDUE LINKERS FORM DIMERS AND WITH ZERO-RESIDUE LINKER A TRIMER
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SINGLE-CHAIN FV FRAGMENTS OF ANTI-NEURAMINIDASE ANTIBODY NC10 CONTAINING FIVE- AND TEN-RESIDUE LINKERS FORM DIMERS AND WITH ZERO-RESIDUE LINKER A TRIMER

机译:含有五残基和十残基连接体的三聚体和零残基连接体的三链抗神经氨酸酶抗体NC10的单链FV片段

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Single-chain variable fragments (scFvs) of anti-neuraminidase antibody NC10 were constructed by joining the V-H and V-L domains with 10-residue (Gly(4)Ser)(2) and five-residue (Gly(4)Ser) linkers; a zero-residue linker scFv was constructed by joining the C-terminal residue of the V-H domain to the N-terminus of the V-L domain. The scFv with the 10- and five-residue linkers exclusively formed dimeric antibody fragments (M-r 52 000), These were shown to be bivalent and were able to cross-link two neuraminidase tetramers to form a 'sandwich' type complex; each antigen combining site could also bind an anti-idiotype Fab'. The zero-residue linker scFv (M-r 70 000) was shown to form a trimer with three active antigen combining sites, each binding an anti-idiotype Fab' to yield a complex of M-r 212 000. The orientation of the combining sites in the zero-residue linker scFv, however, was such that it could not cross-link tetramers of neuraminidase. BIAcore biosensor experiments showed that the affinity of each individual antigen combining site in both the 10- and five-residue linker scFv dimers and zero-residue linker scFv trimer was essentially the same when the scFvs were immobilized onto the sensor surface, However, when the scFvs were used as the analyte, the dimeric and trimeric scFvs showed an apparent increase in binding affinity due to the avidity of binding the multivalent scFvs. [References: 69]
机译:通过将V-H和V-L结构域与10个残基(Gly(4)Ser)(2)和5个残基(Gly(4)Ser)接头连接来构建抗神经氨酸酶抗体NC10的单链可变片段(scFvs);通过将V-H结构域的C-末端残基连接到V-L结构域的N-末端来构建零残基接头scFv。具有10个残基和5个残基的接头的scFv仅形成二聚体抗体片段(M-r 52 000),显示为二价的,能够交联两个神经氨酸酶四聚体形成“三明治”型复合物。每个抗原结合位点也可以结合抗独特型Fab'。零残基接头scFv(Mr 70 000)显示形成具有三个活性抗原结合位点的三聚体,每个结合一个抗独特型Fab'以产生212000 Mr的复合物。结合位点的取向为零然而,残基接头scFv不能与神经氨酸酶的四聚体交联。 BIAcore生物传感器实验表明,当将10个和5个残基的接头scFv二聚体和零残基的接头scFv三聚体固定在传感器表面时,每个单独的抗原结合位点的亲和力基本相同。将scFv用作分析物,由于结合多价scFv的亲和力,二聚和三聚scFv显示出结合亲和力的明显增加。 [参考:69]

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