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葡萄酒和啤酒酵母布鲁塞尔德克酵母CEN1和CEN2的新型着丝粒位点

Novel Centromeric Loci of the Wine and Beer Yeast Dekkera bruxellensis CEN1 and CEN2.

作者信息

Ishchuk Olena P, Vojvoda Zeljko Tanja, Schifferdecker Anna J, Mebrahtu Wisén Sofia, Hagström Åsa K, Rozpędowska Elżbieta, Rørdam Andersen Mikael, Hellborg Linda, Ling Zhihao, Sibirny Andrei A, Piškur Jure

机构信息

Department of Biology, Lund University, Lund, Sweden.

Department of Molecular Genetics and Biotechnology, Institute of Cell Biology, NAS of Ukraine, Lviv, Ukraine.

出版信息

PLoS One. 2016 Aug 25;11(8):e0161741. doi: 10.1371/journal.pone.0161741. eCollection 2016.

Abstract

The wine and beer yeast Dekkera bruxellensis thrives in environments that are harsh and limiting, especially in concentrations with low oxygen and high ethanol. Its different strains' chromosomes greatly vary in number (karyotype). This study isolates two novel centromeric loci (CEN1 and CEN2), which support both the yeast's autonomous replication and the stable maintenance of plasmids. In the sequenced genome of the D. bruxellensis strain CBS 2499, CEN1 and CEN2 are each present in one copy. They differ from the known "point" CEN elements, and their biological activity is retained within ~900-1300 bp DNA segments. CEN1 and CEN2 have features of both "point" and "regional" centromeres: They contain conserved DNA elements, ARSs, short repeats, one tRNA gene, and transposon-like elements within less than 1 kb. Our discovery of a miniature inverted-repeat transposable element (MITE) next to CEN2 is the first report of such transposons in yeast. The transformants carrying circular plasmids with cloned CEN1 and CEN2 undergo a phenotypic switch: They form fluffy colonies and produce three times more biofilm. The introduction of extra copies of CEN1 and CEN2 promotes both genome rearrangements and ploidy shifts, with these effects mediated by homologous recombination (between circular plasmid and genome centromere copy) or by chromosome breakage when integrated. Also, the proximity of the MITE-like transposon to CEN2 could translocate CEN2 within the genome or cause chromosomal breaks, so promoting genome dynamics. With extra copies of CEN1 and CEN2, the yeast's enhanced capacities to rearrange its genome and to change its gene expression could increase its abilities for exploiting new and demanding niches.

摘要

葡萄酒和啤酒酵母布鲁塞尔德克酵母能在恶劣和受限的环境中茁壮生长,尤其是在低氧和高乙醇浓度的环境中。其不同菌株的染色体数量(核型)差异很大。本研究分离出两个新的着丝粒位点(CEN1和CEN2),它们既支持酵母的自主复制,也支持质粒的稳定维持。在布鲁塞尔德克酵母菌株CBS 2499的测序基因组中,CEN1和CEN2各有一个拷贝。它们不同于已知的“点”型着丝粒元件,其生物活性保留在约900 - 1300 bp的DNA片段内。CEN1和CEN2具有“点”型和“区域”型着丝粒的特征:它们在不到1 kb的范围内包含保守的DNA元件、ARSs、短重复序列、一个tRNA基因和转座子样元件。我们在CEN2旁边发现了一个微型反向重复转座元件(MITE),这是酵母中此类转座子的首次报道。携带克隆有CEN1和CEN2的环状质粒的转化体发生表型转换:它们形成蓬松的菌落,生物膜产量增加三倍。额外引入CEN1和CEN2的拷贝会促进基因组重排和倍性变化,这些效应是由同源重组(发生在环状质粒和基因组着丝粒拷贝之间)介导的,或者在整合时由染色体断裂介导。此外,类似MITE的转座子与CEN2的接近可能会使CEN2在基因组内易位或导致染色体断裂,从而促进基因组动态变化。有了额外的CEN1和CEN2拷贝,酵母增强的基因组重排能力和基因表达变化能力可能会增加其开拓新的、苛刻生态位的能力。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/63aa/4999066/8d354bded7d5/pone.0161741.g001.jpg

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