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另外两个用于利什曼原虫稳定转染的独立选择标记。

Two more independent selectable markers for stable transfection of Leishmania.

作者信息

Freedman D J, Beverley S M

机构信息

Department of Biological Chemistry and Molecular Pharmacology, Harvard Medical School, Boston, MA 02115.

出版信息

Mol Biochem Parasitol. 1993 Nov;62(1):37-44. doi: 10.1016/0166-6851(93)90175-w.

Abstract

Genetic transformation of Leishmania has relied upon two exogenous selectable markers, neo and hyg, encoding resistance to G418 and hygromycin B respectively. There is a need for multiple independent selectable markers, since Leishmania is diploid and experimental sexual crosses are not currently feasible. Here we report on the development of two additional markers: pac, conferring resistance to the glycopeptide antibiotic puromycin, and phleo, conferring resistance to the DNA-binding drug phleomycin. We constructed a set of four analogous shuttle vectors with these four markers, using DNA segments flanking the Leishmania major H region hmtxr gene to provide information required for expression. These constructs (pHM-NEO, pHM-HYG, pHM-PAC and pHM-PHLEO) were successfully transfected into L. major, mostly with efficiencies comparable to those observed with previous DHFR-TS-based neo and hyg-containing constructs. The exception was pHM-PHLEO, which transfected 30-fold less efficiently; this may be related to the nonenzymatic mechanism of resistance encoded by phleo. All four constructs were shown to replicate extra-chromosomally. Stable transfectants bearing all paired combinations of pHM constructs were obtained by a second round of transfection. These data show that the four markers are functionally independent and in conjunction with the Leishmania N-acetylglucosaminyl transferase gene, brings the number of selectable markers available in Leishmania to five.

摘要

利什曼原虫的基因转化依赖于两种外源性选择标记,即neo和hyg,它们分别编码对G418和潮霉素B的抗性。由于利什曼原虫是二倍体且目前实验性有性杂交不可行,因此需要多个独立的选择标记。在此,我们报告另外两种标记的开发:pac,赋予对糖肽抗生素嘌呤霉素的抗性;phleo,赋予对DNA结合药物博来霉素的抗性。我们使用利什曼原虫主要H区域hmtxr基因侧翼的DNA片段构建了一组带有这四种标记的四个类似穿梭载体,以提供表达所需的信息。这些构建体(pHM-NEO、pHM-HYG、pHM-PAC和pHM-PHLEO)成功转染到硕大利什曼原虫中,大多数转染效率与先前基于二氢叶酸还原酶-胸苷酸合成酶(DHFR-TS)的含neo和hyg的构建体所观察到的效率相当。例外的是pHM-PHLEO,其转染效率低30倍;这可能与phleo编码的非酶抗性机制有关。所有四个构建体均显示为染色体外复制。通过第二轮转染获得了携带所有pHM构建体配对组合的稳定转染子。这些数据表明这四种标记在功能上是独立的,并且与利什曼原虫N-乙酰葡糖胺基转移酶基因一起,使利什曼原虫中可用的选择标记数量增加到五个。

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