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粗糙脉孢菌中由异型序列和减数分裂沉默控制的重组热点。

Recombination hotspots in Neurospora crassa controlled by idiomorphic sequences and meiotic silencing.

机构信息

College of Science and Engineering, Flinders University, Sturt Road, Bedford Park, South Australia 5042, Australia.

出版信息

Genetics. 2024 Feb 7;226(2). doi: 10.1093/genetics/iyad213.

DOI:10.1093/genetics/iyad213
PMID:38124387
Abstract

Genes regulating recombination in specific chromosomal intervals of Neurospora crassa were described in the 1960s, but the mechanism is still unknown. For each of the rec-1, rec-2, and rec-3 genes, a single copy of the putative dominant allele, for example, rec-2SL found in St Lawrence OR74 A wild type, reduces recombination in chromosomal regions specific to that gene. However, when we sequenced the recessive allele, rec-2LG (derived from the Lindegren 1A wild type), we found that a 10 kb region in rec-2SL strains was replaced by a 2.7 kb unrelated sequence, making the "alleles" idiomorphs. When we introduced sad-1, a mutant lacking the RNA-dependent RNA polymerase that silences unpaired coding regions during meiosis into crosses heterozygous rec-2SL/rec-2LG, it increased recombination, indicating that meiotic silencing of a gene promoting recombination is responsible for dominant suppression of recombination. Consistent with this, mutation of rec-2LG by Repeat-Induced Point mutation generated an allele with multiple stop codons in the predicted rec-2 gene, which does not promote recombination and is recessive to rec-2LG. Sad-1 also relieves suppression of recombination in relevant target regions, in crosses heterozygous for rec-1 alleles and in crosses heterozygous for rec-3 alleles. We conclude that for all 3 known rec genes, 1 allele appears dominant only because meiotic silencing prevents the product of the active, "recessive," allele from stimulating recombination during meiosis. In addition, the proposed amino acid sequence of REC-2 suggests that regulation of recombination in Neurospora differs from any currently known mechanism.

摘要

20 世纪 60 年代描述了调控粗糙脉孢菌特定染色体间隔重组的基因,但该机制仍不清楚。对于每个 rec-1、rec-2 和 rec-3 基因,一个假定的显性等位基因的单一拷贝,例如 St Lawrence OR74A 野生型中的 rec-2SL,会降低与该基因特异性相关的染色体区域的重组。然而,当我们对隐性等位基因 rec-2LG(源自 Lindegren 1A 野生型)进行测序时,我们发现 rec-2SL 菌株中的 10kb 区域被一个 2.7kb 的不相关序列取代,使“等位基因”成为同形物。当我们将缺乏 RNA 依赖性 RNA 聚合酶的突变体 sad-1(该酶在减数分裂期间沉默未配对的编码区)引入到杂合 rec-2SL/rec-2LG 的杂交中时,它增加了重组,表明促进重组的基因的减数沉默是显性抑制重组的原因。这与重复诱导点突变突变 rec-2LG 产生的一个等位基因一致,该等位基因在预测的 rec-2 基因中具有多个终止密码子,不能促进重组,且对 rec-2LG 为隐性。Sad-1 还缓解了在相关靶区域中重组的抑制,在杂合 rec-1 等位基因的杂交和杂合 rec-3 等位基因的杂交中均如此。我们得出结论,对于所有 3 个已知的 rec 基因,一个等位基因似乎是显性的,仅仅是因为减数沉默阻止了活性的“隐性”等位基因的产物在减数分裂期间刺激重组。此外,所提出的 REC-2 氨基酸序列表明,粗糙脉孢菌的重组调控与任何当前已知的机制都不同。

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Recombination hotspots in Neurospora crassa controlled by idiomorphic sequences and meiotic silencing.粗糙脉孢菌中由异型序列和减数分裂沉默控制的重组热点。
Genetics. 2024 Feb 7;226(2). doi: 10.1093/genetics/iyad213.
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Occurrence in wild strains of Neurospora crassa of genes controlling genetic recombination.粗糙脉孢菌野生菌株中控制基因重组的基因的出现。
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Evidence for the absence of meiotic silencing by unpaired DNA in Neurospora tetrasperma.关于四孢链孢霉中未配对DNA不存在减数分裂沉默的证据。
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Chromosome segment duplications in Neurospora crassa and their effects on repeat-induced point mutation and meiotic silencing by unpaired DNA.粗糙脉孢菌中的染色体片段重复及其对重复序列诱导点突变和未配对DNA引发的减数分裂沉默的影响。
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Fluorescent Protein as a Tool for Investigating Meiotic Recombination in Neurospora.荧光蛋白作为研究粗糙脉孢菌减数分裂重组的工具
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