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大肠杆菌原生质体的转染。3. 不同碱性聚合物对转染的促进作用及原生质体的稳定作用

Transfection of Escherichia coli spheroplasts. 3. Facilitation of transfection and stabilization of spheroplasts by different basic polymers.

作者信息

Henner W D, Kleber I, Benzinger R

出版信息

J Virol. 1973 Oct;12(4):741-7. doi: 10.1128/JVI.12.4.741-747.1973.

Abstract

The only compound which fully replaced protamine sulfate in facilitating transfection of Escherichia coli spheroplasts by phage DNAs was spermine; poly-l-lysine, poly-l-arginine, DEAE-dextran, histones, and many other polyamines were only slightly effective. Higher-molecular-weight compounds were effective at lower concentrations, and each compound had a sharp concentration optimum. The specificity of the facilitation of transfection is discussed in light of Leonard and Cole's (1972) isolation of a polyamine- or protamine-like, natural competence factor from Streptococci. By standardizing growth conditions for spheroplast cultures, storing spheroplasts in minimal medium, and adding both protamine sulfate and polyamines to spheroplasts, reproducible competence levels were obtained. Thus, 95% of all spheroplast preparations gave efficiencies of transfection between 10(-3) and 3 x 10(-4) for lambda DNA; between 10(-6) and 3 x 10(-8) for T7 DNA; and between 3 x 10(-6) and 10(-7) for T5 phage DNA. The stability of the spheroplasts was extended from 10 h to between 2 and 5 days, depending on the DNA used for transfection.

摘要

在促进噬菌体DNA转染大肠杆菌原生质球方面,唯一能完全替代硫酸鱼精蛋白的化合物是精胺;聚-L-赖氨酸、聚-L-精氨酸、二乙氨基乙基葡聚糖、组蛋白以及许多其他多胺的效果都很微弱。分子量较高的化合物在较低浓度下有效,且每种化合物都有一个明显的最佳浓度。根据伦纳德和科尔(1972年)从链球菌中分离出一种多胺或鱼精蛋白样的天然感受态因子,对转染促进作用的特异性进行了讨论。通过规范原生质球培养的生长条件,将原生质球保存在基本培养基中,并向原生质球中添加硫酸鱼精蛋白和多胺,获得了可重复的感受态水平。因此,所有原生质球制备物中,95%对λDNA的转染效率在10^(-3)至3×10^(-4)之间;对T7 DNA的转染效率在10^(-6)至3×10^(-8)之间;对T5噬菌体DNA的转染效率在3×10^(-6)至10^(-7)之间。原生质球的稳定性从10小时延长至2至5天,这取决于用于转染的DNA。

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