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通过电穿孔法制备的转基因斑马鱼中RSVCAT的瞬时表达。

Transient expression of RSVCAT in transgenic zebrafish made by electroporation.

作者信息

Buono R J, Linser P J

机构信息

Whitney Marine Laboratory, University of Florida, St. Augustine 32086.

出版信息

Mol Mar Biol Biotechnol. 1992 Aug-Oct;1(4-5):271-5.

PMID:1339227
Abstract

We report the fish use of an exponential decay electroporation system to introduce foreign DNA into fertilized zebrafish embryos. The plasmid RSVCAT (Rous sarcoma viral promoter (RSV) upstream from the chloramphenicol acetyltransferase gene (CAT)) was linearized and introduced into fertile zebrafish embryos by electroporation no later than the four-cell stage. Conditions for the procedure were empirically derived, and 68% of the treated animals survived through hatching to at least 6 days after fertilization and well beyond. Dot-blot analysis on DNA extracted from individual hatching fry demonstrated that 65% of the animals tested carried the foreign construct. Enzyme assays on the soluble proteins of treated animals were positive for chloramphenicol acetyltransferase activity. These data demonstrate that the foreign construct was being transiently expressed in the developing tissues of the embryo. The simplicity of this technique will greatly enhance the ability to analyze gene promoter regulation in vivo in transgenic zebrafish. The ability of the electroporated DNA to integrate into the host genome and to generate stable lines of transgenic fish is discussed.

摘要

我们报道了利用指数衰减电穿孔系统将外源DNA导入受精斑马鱼胚胎的实验。质粒RSVCAT(氯霉素乙酰转移酶基因(CAT)上游的劳氏肉瘤病毒启动子(RSV))被线性化,并在不晚于四细胞期时通过电穿孔导入可育斑马鱼胚胎。该实验步骤的条件是通过经验得出的,68%的处理过的动物存活至孵化后至少6天,甚至更久。对从单个孵化幼鱼中提取的DNA进行斑点印迹分析表明,65%的受试动物携带外源构建体。对处理过的动物的可溶性蛋白进行酶分析,结果显示氯霉素乙酰转移酶活性呈阳性。这些数据表明,外源构建体在胚胎发育组织中短暂表达。这项技术的简便性将大大增强在转基因斑马鱼体内分析基因启动子调控的能力。本文还讨论了电穿孔DNA整合到宿主基因组并产生稳定转基因鱼系的能力。

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