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多细胞绿藻团藻的基因工程:一个经过修饰和倍增的细菌抗生素抗性基因作为显性选择标记

Genetic engineering of the multicellular green alga Volvox: a modified and multiplied bacterial antibiotic resistance gene as a dominant selectable marker.

作者信息

Hallmann A, Rappel A

机构信息

Lehrstuhl Biochemie I, Universität Regensburg, Germany.

出版信息

Plant J. 1999 Jan;17(1):99-109. doi: 10.1046/j.1365-313x.1999.00342.x.

Abstract

The green alga Volvox represents the simplest multicellular organism: Volvax is composed of only two cell types, somatic and reproductive. Volvox, therefore, is an attractive model system for studying various aspects of multicellularity. With the biolistic nuclear transformation of Volvox carteri, the powerful molecular genetic manipulation of this organism has been established, but applications have been restricted to an auxotrophic mutant serving as the DNA recipient. Therefore, a dominant selectable marker working in all strains and mutants of this organism is required. Among several gene constructs tested, the most advantageous results were obtained with a chimeric gene composed of the coding sequence of the bacterial ble gene, conferring resistance to the antibiotic zeocin, modified with insertions of two endogenous introns from the Volvox arylsulfatase gene and fused to 5' and 3' untranslated regions from the Volvox beta 2-tubulin gene. In the most suitable plasmid used, the gene dosage was increased 16-fold by a technique that allows exponential multiplication of a DNA fragment. Co-transformation of this plasmid and a non-selectable plasmid allowed the identification of zeocin resistant transformants with nuclear integration of both selectable and non-selectable plasmids. Stable expression of the ble gene and of genes from several non-selectable plasmids is demonstrated. The modified ble gene provides the first dominant marker for transformation of both wild-type and mutant strains of Volvox.

摘要

绿藻团藻是最简单的多细胞生物

团藻仅由两种细胞类型组成,即体细胞和生殖细胞。因此,团藻是研究多细胞性各个方面的一个有吸引力的模型系统。通过对卡特团藻进行生物弹道核转化,已建立了对该生物体强大的分子遗传操作,但应用仅限于以营养缺陷型突变体作为DNA受体。因此,需要一种在该生物体的所有菌株和突变体中都能起作用的显性选择标记。在测试的几种基因构建体中,由细菌ble基因的编码序列组成的嵌合基因获得了最有利的结果,该基因赋予对博来霉素的抗性,通过插入来自团藻芳基硫酸酯酶基因的两个内源性内含子进行修饰,并与来自团藻β2-微管蛋白基因的5'和3'非翻译区融合。在使用的最合适的质粒中,通过一种允许DNA片段指数增殖的技术,基因剂量增加了16倍。该质粒与一个非选择性质粒的共转化使得能够鉴定出同时整合了选择性质粒和非选择性质粒的博来霉素抗性转化体。证明了ble基因和几种非选择性质粒中的基因的稳定表达。修饰后的ble基因提供了第一个用于团藻野生型和突变体菌株转化的显性标记。

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