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小鼠B淋巴细胞抗DNA库的克隆分析。

Clonal analysis of the anti-DNA repertoire of murine B lymphocytes.

作者信息

Conger J D, Pike B L, Nossal G J

出版信息

Proc Natl Acad Sci U S A. 1987 May;84(9):2931-5. doi: 10.1073/pnas.84.9.2931.

DOI:10.1073/pnas.84.9.2931
PMID:3495004
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC304774/
Abstract

The present studies characterize at the clonal level the repertoire of lipopolysaccharide-responsive murine B lymphocytes committed to the production of antibodies reactive with denatured DNA. This repertoire is vast in normal mice as 1-5% of total mitogen-induced antibody-forming cell clones secreted denatured DNA-reactive antibodies when the splenocyte donors were CBA (Ighj), BALB/c (Igha), C57BL/6 (Ighb), CBA nu/nu, and C57BL/6 nu/nu athymic mice. The autoimmune NZB (Ighe) strain did not display elevated proportions of anti-denatured DNA antibody-forming cell precursors. Cross-reactions shown by CBA anti-denatured DNA antibodies suggest that many antibodies might derive significant binding energy from interaction with the bases or similar hydrophobic moieties. Cross-reactions with other tested polynucleotides were frequent, but cross-reactions with phospholipids and phosphocholine were undetectable. Most anti-DNA antibodies bound preferentially or exclusively to single-stranded denatured DNA as compared to double-stranded native DNA. The frequency of anti-denatured DNA antibody-forming cell precursors among CBA peritoneal cells was not elevated. Fluorescence-activated cell sorter-selected Ly-1-positive NZB splenic B cells were not enriched, and Ly-1 negative B cells were not depleted of anti-DNA antibody-forming cell precursors. These results show that antibody-forming cell precursors specific for denatured DNA are not restricted to the Ly-1 positive B-cell subset.

摘要

本研究在克隆水平上对脂多糖反应性小鼠B淋巴细胞的谱系进行了表征,这些B淋巴细胞致力于产生与变性DNA反应的抗体。在正常小鼠中,该谱系极为广泛,因为当脾细胞供体为CBA(Ighj)、BALB/c(Igha)、C57BL/6(Ighb)、CBA裸鼠和C57BL/6裸鼠无胸腺小鼠时,有1%-5%的丝裂原诱导的抗体形成细胞克隆分泌与变性DNA反应的抗体。自身免疫性NZB(Ighe)品系未显示出抗变性DNA抗体形成细胞前体比例的升高。CBA抗变性DNA抗体所显示的交叉反应表明,许多抗体可能从与碱基或类似疏水基团的相互作用中获得显著的结合能。与其他测试的多核苷酸的交叉反应很常见,但与磷脂和磷酸胆碱的交叉反应未检测到。与双链天然DNA相比,大多数抗DNA抗体优先或仅与单链变性DNA结合。CBA腹膜细胞中抗变性DNA抗体形成细胞前体的频率未升高。荧光激活细胞分选仪选择的Ly-1阳性NZB脾B细胞未富集,Ly-1阴性B细胞也未耗尽抗DNA抗体形成细胞前体。这些结果表明,对变性DNA特异的抗体形成细胞前体不限于Ly-1阳性B细胞亚群。

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本文引用的文献

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