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构建用于染色体介导基因转移的、在小鼠17号染色体上含有不同新基因插入片段的微细胞杂交板。

Construction of microcell hybrid panel containing different neo gene insertions in mouse chromosome 17 used for chromosome-mediated gene transfer.

作者信息

Sidén T S, Höglund M, Röhme D

机构信息

Department of Molecular Genetics, University of Lund, Sweden.

出版信息

Somat Cell Mol Genet. 1989 May;15(3):245-53. doi: 10.1007/BF01534875.

Abstract

A panel of four microcell hybrids representing different sites of insertion of the exogenous neo gene into mouse chromosome 17 has been constructed. These constructions were based on a cotransfer of mouse chromosome 17 and neomycin resistance generated in a stepwise procedure involving (1) random insertion of the neo gene into a primary cell hybrid containing mouse chromosome 17 in a hamster cell background, (2) microcell-mediated chromosome transfer (MMCT) to segregate mouse and hamster chromosomes, and (3) identification of the mouse chromosome containing cells using a novel cell dotting procedure for mass screening at the cell colony level by molecular hybridization. Using this panel of four microcell hybrids for chromosome mediated gene transfer (CMGT), we obtained one transformant containing a chromosome fragment derived from the t-complex region located on mouse chromosome 17. It is concluded that the specific chromosome based procedure used here to generate CMGT transfectants may provide a general means to produce large numbers of transfectants containing megabase fragments covering, in principle, all regions of a given chromosome.

摘要

构建了一组四个微细胞杂种,它们代表外源新霉素基因插入小鼠17号染色体的不同位点。这些构建基于小鼠17号染色体和新霉素抗性的共转移,该过程分步骤进行,包括:(1)将新霉素基因随机插入仓鼠细胞背景下含有小鼠17号染色体的原代细胞杂种中;(2)微细胞介导的染色体转移(MMCT)以分离小鼠和仓鼠染色体;(3)通过分子杂交在细胞集落水平进行大规模筛选的新型细胞点样程序来鉴定含有小鼠染色体的细胞。使用这组四个微细胞杂种进行染色体介导的基因转移(CMGT),我们获得了一个转化体,其含有源自位于小鼠17号染色体上的t-复合体区域的染色体片段。结论是,这里用于产生CMGT转染子的基于特定染色体的程序可能提供一种通用方法,以产生大量含有原则上覆盖给定染色体所有区域的兆碱基片段的转染子。

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