Rapid cloning of mammalian cells with honeycomb cloning plates and nonlethal vital stains.

In Vitro Pub Date : 1984-02-01 DOI:10.1007/BF02626653
R J Klebe
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引用次数: 1

Abstract

A rapid and technically simple method for cloning both adhesive and nonadhesive mammalian cells is described. The procedure employs (a) honeycomb cloning plates and (b) nonlethal vital stains. Instead of placing cloning rings around colonies, cells are initially seeded at clonal density directly into a plate containing an array of cloning rings (the honeycomb plate). Hence, the time involved in placing cloning rings around colonies is eliminated. Second, clone-containing wells of the honeycomb plate are easily identified by staining plates with the nonlethal vital stains, MTT or INT tetrazolium. Vital staining eliminates the time involved in searching for clones. Last, clones are transferred with a cotton-tipped swab thereby eliminating the time involved in trypsinization of cells. In this fashion, one can pick and transfer clones of substrate adherent mammalian cells at a rate of one clone/10 to 15 s. Thus, mammalian cells can be cloned as rapidly as cloning can be carried out in microbial systems.

用蜂窝克隆板和非致命的活体染色快速克隆哺乳动物细胞。
描述了一种快速和技术上简单的克隆粘附和非粘附哺乳动物细胞的方法。该程序采用(a)蜂窝克隆板和(b)非致命的生命染色。不是在菌落周围放置克隆环,而是首先按克隆密度将细胞直接播种到含有克隆环阵列的板(蜂窝板)中。因此,消除了在菌落周围放置克隆环的时间。其次,用非致死性生命染色剂MTT或INT四氮唑对蜂窝板进行染色,可以很容易地识别蜂窝板的克隆孔。活体染色消除了寻找克隆的时间。最后,用棉签转移克隆,从而消除了细胞胰蛋白酶化所涉及的时间。在这种方式下,人们可以以每10到15秒一个克隆的速度挑选和转移底物粘附的哺乳动物细胞的克隆。因此,克隆哺乳动物细胞的速度与克隆微生物细胞的速度一样快。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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