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一种通过转基因实现雄性生殖细胞介导基因传递的非手术方法。

A non-surgical approach for male germ cell mediated gene transmission through transgenesis.

作者信息

Usmani Abul, Ganguli Nirmalya, Sarkar Hironmoy, Dhup Suveera, Batta Suryaprakash R, Vimal Manoj, Ganguli Nilanjana, Basu Sayon, Nagarajan P, Majumdar Subeer S

机构信息

Embryo Biotechnology Laboratory, National Institute of Immunology, New Delhi, India.

出版信息

Sci Rep. 2013 Dec 5;3:3430. doi: 10.1038/srep03430.

Abstract

Microinjection of foreign DNA in male pronucleus by in-vitro embryo manipulation is difficult but remains the method of choice for generating transgenic animals. Other procedures, including retroviral and embryonic stem cell mediated transgenesis are equally complicated and have limitations. Although our previously reported technique of testicular transgenesis circumvented several limitations, it involved many steps, including surgery and hemicastration, which carried risk of infection and impotency. We improved this technique further, into a two step non-surgical electroporation procedure, for making transgenic mice. In this approach, transgene was delivered inside both testes by injection and modified parameters of electroporation were used for in-vivo gene integration in germ cells. Using variety of constructs, germ cell integration of the gene and its transmission in progeny was confirmed by PCR, slot blot and immunohistochemical analysis. This improved technique is efficient, requires substantially less time and can be easily adopted by various biomedical researchers.

摘要

通过体外胚胎操作将外源DNA显微注射到雄原核中虽然困难,但仍然是生成转基因动物的首选方法。其他方法,包括逆转录病毒和胚胎干细胞介导的转基因同样复杂且存在局限性。尽管我们之前报道的睾丸转基因技术规避了一些局限性,但它涉及多个步骤,包括手术和半阉割,存在感染和阳痿的风险。我们进一步改进了该技术,将其转变为两步非手术电穿孔程序来制作转基因小鼠。在这种方法中,通过注射将转基因导入双侧睾丸,并使用改良的电穿孔参数在生殖细胞中进行体内基因整合。通过PCR、狭缝印迹和免疫组织化学分析,使用多种构建体证实了基因在生殖细胞中的整合及其在后代中的传递。这种改进后的技术效率高,所需时间大大减少,并且各种生物医学研究人员都可以轻松采用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/69c3/3852150/8f2c5346c081/srep03430-f1.jpg

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