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实验室保藏的热带利什曼原虫中的扩增DNA:染色体外环状结构,在结构和功能上与耐甲氨蝶呤的硕大利什曼原虫的倒H区扩增相似。

Amplified DNAs in laboratory stocks of Leishmania tarentolae: extrachromosomal circles structurally and functionally similar to the inverted-H-region amplification of methotrexate-resistant Leishmania major.

作者信息

Petrillo-Peixoto M L, Beverley S M

机构信息

Department of Biological Chemistry and Molecular Pharmacology, Harvard Medical School, Boston, Massachusetts 02115.

出版信息

Mol Cell Biol. 1988 Dec;8(12):5188-99. doi: 10.1128/mcb.8.12.5188-5199.1988.

Abstract

We describe the structure of amplified DNA that was discovered in two laboratory stocks of the protozoan parasite Leishmania tarentolae. Restriction mapping and molecular cloning revealed that a region of 42 kilobases was amplified 8- to 30-fold in these lines. Southern blot analyses of digested DNAs or chromosomes separated by pulsed-field electrophoresis showed that the amplified DNA corresponded to the H region, a locus defined originally by its amplification in methotrexate-resistant Leishmania major (S. M. Beverley, J. A. Coderre, D. V. Santi, and R. T. Schimke, Cell 38:431-439, 1984). Similarities between the amplified DNA of the two species included (i) extensive cross-hybridization; (ii) approximate conservation of sequence order; (iii) extrachromosomal localization; (iv) an overall inverted, head-to-head configuration as a circular 140-kilobase tetrameric molecule; (v) two regions of DNA sequence rearrangement, each of which was closely associated with the two centers of the inverted repeats; (vi) association with methotrexate resistance; and (vii) phenotypically conservative amplification, in which the wild-type chromosomal arrangement was retained without apparent modification. Our data showed that amplified DNA mediating drug resistance arose in unselected L. tarentolae, although the pressures leading to apparently spontaneous amplification and maintenance of the H region are not known. The simple structure and limited extent of DNA amplified in these and other Leishmania lines suggests that the study of gene amplification in Leishmania spp. offers an attractive model system for the study of amplification in cultured mammalian cells and tumors. We also introduced a method for measuring the size of large circular DNAs, using gamma-irradiation to introduce limited double-strand breaks followed by sizing of the linear DNAs by pulsed-field electrophoresis.

摘要

我们描述了在原生动物寄生虫塔兰托拉利什曼原虫的两个实验室菌株中发现的扩增DNA的结构。限制性图谱分析和分子克隆表明,在这些品系中,一个42千碱基的区域被扩增了8至30倍。对通过脉冲场电泳分离的消化DNA或染色体进行的Southern印迹分析表明,扩增的DNA对应于H区域,该位点最初是通过其在抗甲氨蝶呤的硕大利什曼原虫中的扩增而定义的(S.M.贝弗利、J.A.科德雷、D.V.桑蒂和R.T.希姆克,《细胞》38:431 - 439,1984)。这两个物种的扩增DNA之间的相似性包括:(i)广泛的交叉杂交;(ii)序列顺序大致保守;(iii)染色体外定位;(iv)作为一个140千碱基的环状四聚体分子的整体反向、头对头构型;(v)两个DNA序列重排区域,每个区域都与反向重复的两个中心紧密相关;(vi)与甲氨蝶呤抗性相关;(vii)表型保守扩增,其中野生型染色体排列得以保留而无明显修饰。我们的数据表明,介导耐药性的扩增DNA出现在未选择的塔兰托拉利什曼原虫中,尽管导致H区域明显自发扩增和维持的压力尚不清楚。在这些以及其他利什曼原虫品系中扩增的DNA的简单结构和有限范围表明,对利什曼原虫属基因扩增的研究为研究培养的哺乳动物细胞和肿瘤中的扩增提供了一个有吸引力的模型系统。我们还介绍了一种测量大型环状DNA大小的方法,即使用γ射线照射引入有限的双链断裂,然后通过脉冲场电泳对线性DNA进行大小测定。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/fde1/365621/218f8bd6ac43/molcellb00072-0142-a.jpg

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