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一种极低密度原生质体显微注射和培养的方法。

A method for the microinjection and culture of protoplasts at very low densities.

机构信息

John Innes Institute, Colney Lane, NR4 7UH, Norwich, UK.

出版信息

Plant Cell Rep. 1985 Feb;4(1):33-5. doi: 10.1007/BF00285500.

Abstract

A method has been developed which allows the recovery of calli from a high proportion of individual, injected, mesophyll protoplasts of Nicotiana tabacum c.v. Xanthi. A small drop of low melting point agarose is used both to hold protoplasts during microinjection and for their subsequent culture in feeder dishes. The feeder dishes consist of "beads" of protoplasts at a high density set in agarose to "feed" the infected protoplasts across a liquid medium.The method has been used successfully both with normal protoplasts and protoplasts from which the vacuole has been removed.

摘要

已经开发出一种方法,该方法允许从大量单个、注射的烟草中叶原生质体中回收愈伤组织。在微量注射过程中,使用一小滴低熔点琼脂糖来固定原生质体,并在饲养盘中进行后续培养。饲养盘由高浓度的“珠状”原生质体组成,置于琼脂糖中,以便在液体培养基中“喂养”感染的原生质体。该方法已成功用于正常原生质体和去除液泡的原生质体。

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