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Identification of two aberrant transcripts derived from a hybridoma with amplification of functional immunoglobulin variable genes

机译:鉴定源自杂交瘤的两个异常转录本并扩增功能性免疫球蛋白可变基因

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摘要

Murine monoclonal antibodies (mAbs) are widely used but have limitations if administered in humans. The use of chimeric or humanized mAbs can reduce immunogenicity. The first step in producing such mAbs is to clone murine variable genes from a hybridoma, but it is possible to amplify both functional and aberrant variable genes, as they coexist in the hybridoma. During the development of a murine–human chimeric antibody, we have cloned from a hybridoma the functional heavy chain variable region (VH) and light chain variable region (VL) genes of a mAb that blocks the binding of anthrax lethal factor to protective antigen. In this study, we report the detection of two aberrant transcripts from a hybridoma produced using myeloma cell line OUR-1, the development of a method to distinguish between the functional and abundant aberrant VL transcripts, and the origins of these aberrant genes. The aberrant VL gene is derived from OUR-1 cells, while the aberrant VH gene might derive from antibody repertoires in B cells or from gene rearrangement in the hybridoma cells. The aberrant VH and VL genes in this study may facilitate discrimination between the functional and aberrant variable genes from hybridoma cells.
机译:鼠单克隆抗体(mAb)被广泛使用,但如果在人体中施用则具有局限性。嵌合或人源化单克隆抗体的使用可降低免疫原性。产生此类mAb的第一步是从杂交瘤中克隆鼠类可变基因,但是有可能同时扩增功能性和异常可变基因,因为它们共存于杂交瘤中。在鼠-人嵌合抗体的开发过程中,我们从杂交瘤中克隆了单克隆抗体的功能性重链可变区(VH)和轻链可变区(VL)基因,可阻断炭疽致死因子与保护性抗原的结合。在这项研究中,我们报告了从使用骨髓瘤细胞系OUR-1产生的杂交瘤中检测到两个异常转录本,开发了一种区分功能性和丰富异常VL转录本的方法,以及这些异常基因的起源。异常的VL基因源自OUR-1细胞,而异常的VH基因可能源自B细胞中的抗体库或杂交瘤细胞中的基因重排。这项研究中异常的VH和VL基因可能有助于区分杂交瘤细胞的功能性和异常可变基因。

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