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曼氏血吸虫:利用克隆的核糖体RNA基因探针检测中间宿主光滑双脐螺中的限制性片段长度多态性。

Schistosoma mansoni: use of a cloned ribosomal RNA gene probe to detect restriction fragment length polymorphisms in the intermediate host Biomphalaria glabrata.

作者信息

Knight M, Brindley P J, Richards C S, Lewis F A

机构信息

Biomedical Research Institute, Rockville, Maryland 20852.

出版信息

Exp Parasitol. 1991 Oct;73(3):285-94. doi: 10.1016/0014-4894(91)90100-b.

DOI:10.1016/0014-4894(91)90100-b
PMID:1680745
Abstract

Adult susceptibility of Biomphalaria glabrata to Schistosoma mansoni infection is controlled by simple Mendelian genetics. In this study a molecular approach was used to determine the degree of genetic variation between well-defined lines of B. glabrata which are either resistant (10-R2) or susceptible (M-line) to S. mansoni infection. A cloned probe pSM389, which contains part of the S. mansoni small ribosomal RNA gene and a portion of the nontranscribed spacer was found to cross-hybridize with B. glabrata DNA and was used in Southern hybridizations to detect restriction fragment length polymorphisms (RFLPs) between the above snail stocks. Polymorphisms were noted with a variety of restriction enzymes, namely Bg/II, BamHI, AccI, AvaII, ClaI, EcoRI, EcoRV, KpnI, PvuII, and NcoI. Although most RFLPs were relatively minor, a significant difference was observed with EcoRV. Further analysis of the EcoRV RFLPs among other isolates of the resistant stock demonstrated that a high frequency of genetic variation exists even among isolates of the same origin, but maintained in separate laboratories. Interestingly, RFLPs in the EcoRV site were detected in DNA isolated from a single generation of selfed progeny of a single 10-R2 parent. RFLPs associated with this site were found to occur between B. glabrata and B. tenagophila, B. straminea, and B. schrammi, indicating that Southern blot analysis using ribosomal gene probes may be useful for the molecular differentiation of B. glabrata from other intermediate hosts and from morphologically similar species that are refractory to infection.

摘要

光滑双脐螺对曼氏血吸虫感染的成体易感性受简单孟德尔遗传学控制。在本研究中,采用分子方法来确定光滑双脐螺明确品系之间的遗传变异程度,这些品系对曼氏血吸虫感染分别具有抗性(10-R2)或易感性(M系)。发现一个克隆探针pSM389,其包含曼氏血吸虫小核糖体RNA基因的一部分和非转录间隔区的一部分,可与光滑双脐螺DNA发生交叉杂交,并用于Southern杂交以检测上述螺类种群之间的限制性片段长度多态性(RFLP)。使用多种限制性内切酶,即Bg/II、BamHI、AccI、AvaII、ClaI、EcoRI、EcoRV、KpnI、PvuII和NcoI时,均观察到多态性。尽管大多数RFLP相对较小,但使用EcoRV时观察到显著差异。对抗性种群其他分离株之间的EcoRV RFLP进行进一步分析表明,即使在同一来源的分离株之间也存在高频遗传变异,不过这些分离株保存在不同实验室中。有趣的是,在从单个10-R2亲本的单代自交后代中分离的DNA中检测到EcoRV位点的RFLP。发现与该位点相关的RFLP存在于光滑双脐螺与嗜气管双脐螺、稻草双脐螺和施氏双脐螺之间,这表明使用核糖体基因探针进行Southern印迹分析可能有助于从其他中间宿主以及从形态相似但对感染有抗性的物种中对光滑双脐螺进行分子鉴别。

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