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Molecular mechanism for generation of antibody memory

机译:抗体记忆产生的分子机制

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Activation-induced cytidine deaminase ( AID) is the essential enzyme inducing the DNA cleavage required for both somatic hypermutation and class switch recombination (CSR) of the immunoglobulin gene. We originally proposed the RNA-editing model for the mechanism of DNA cleavage by AID. We obtained evidence that fulfils three requirements for CSR by this model, namely (i) AID shuttling between nucleus and cytoplasm, (ii) de novo protein synthesis for CSR, and (iii) AID-RNA complex formation. The alternative hypothesis, designated as the DNA-deamination model, assumes that the in vitro DNA deamination activity of AID is representative of its physiological function in vivo. Furthermore, the resulting dU was removed by uracil DNA glycosylase (UNG) to generate a basic site, followed by phosphodiester bond cleavage by AP endonuclease. We critically examined each of these provisional steps. We identified a cluster of mutants (H48A, L49A, R50A and N51A) that had particularly higher CSR activities than expected from their DNA deamination activities. The most striking was the N51A mutant that had no ability to deaminate DNA in vitro but retained approximately 50 per cent of the wild-type level of CSR activity. We also provide further evidence that UNG plays a non-canonical role in CSR, namely in the repair step of the DNA breaks. Taking these results together, we favour the RNA-editing model for the function of AID in CSR.
机译:激活诱导的胞苷脱氨酶(AID)是诱导免疫球蛋白基因的体细胞超突变和类开关重组(CSR)所需的DNA切割的必需酶。我们最初提出了用于通过AID进行DNA切割的机制的RNA编辑模型。我们获得了满足该模型对CSR的三个要求的证据,即(i)AID在核和细胞质之间穿梭,(ii)CSR从头合成蛋白质,以及(iii)AID-RNA复合物形成。称为DNA脱氨模型的另一种假设假设AID的体外DNA脱氨活性代表其体内的生理功能。此外,通过尿嘧啶DNA糖基化酶(UNG)去除所得的dU以产生碱性位点,然后通过AP核酸内切酶切割磷酸二酯键。我们严格审查了这些临时步骤。我们鉴定了一组突变体(H48A,L49A,R50A和N51A),它们的CSR活性比其DNA脱氨活性预期的要特别高。最引人注目的是N51A突变体,该突变体无法在体外使DNA脱氨,但是保留了野生型CSR活性水平的大约50%。我们还提供了进一步的证据,证明UNG在CSR(即DNA断裂的修复步骤)中起着非典型的作用。综合这些结果,我们赞成AID在CSR中的功能的RNA编辑模型。

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