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Zfs1p 对裂殖酵母细胞间相互作用蛋白编码转录本的转录后调控。

Posttranscriptional regulation of cell-cell interaction protein-encoding transcripts by Zfs1p in Schizosaccharomyces pombe.

机构信息

Laboratory of Signal Transduction, National Institute of Environmental Health Sciences, Research Triangle Park, North Carolina, USA.

出版信息

Mol Cell Biol. 2012 Oct;32(20):4206-14. doi: 10.1128/MCB.00325-12. Epub 2012 Aug 20.

Abstract

Members of the tristetraprolin (TTP) family of CCCH tandem zinc finger proteins can bind directly to AU-rich elements in mRNAs and promote transcript deadenylation and decay. The yeast Schizosaccharomyces pombe expresses a single TTP family member, Zfs1p. In this study, we identified probable Zfs1p target mRNAs by comparing transcript levels in wild-type yeast and zfs1Δ mutants, using deep sequencing and microarray approaches. We also used direct RNA sequencing to determine polyadenylation site locations and to confirm the presence of potential Zfs1p target sequences within the target mRNA. These studies identified a set of transcripts containing potential Zfs1p binding sites that accumulated significantly in the zfs1Δ mutants; a subset of these transcripts decayed more slowly in the zfs1Δ mutants and bound directly to Zfs1p in coimmunoprecipitation assays. One apparent direct target encodes the transcription factor Cbf12p, which is known to increase cell-cell adhesion and flocculation when overexpressed. Studies of zfs1Δ cbf12Δ double mutants demonstrated that the increased flocculation seen in zfs1Δ mutants is due, at least in part, to a direct effect on the turnover of cbf12 mRNA. These data suggest that Zfs1p can both directly and indirectly regulate the levels of transcripts involved in cell-cell adhesion in this species.

摘要

Tristetraprolin(TTP)家族的 CCCH 串联锌指蛋白成员可以直接结合 mRNA 中的 AU 丰富元件,并促进转录物的脱腺苷酸化和降解。酵母酿酒酵母表达单个 TTP 家族成员 Zfs1p。在这项研究中,我们通过比较野生型酵母和 zfs1Δ 突变体中的转录水平,使用深度测序和微阵列方法,鉴定了可能的 Zfs1p 靶 mRNA。我们还使用直接 RNA 测序来确定多聚腺苷酸化位点的位置,并在靶 mRNA 中确认存在潜在的 Zfs1p 靶序列。这些研究确定了一组包含潜在 Zfs1p 结合位点的转录本,这些转录本在 zfs1Δ 突变体中显著积累;这些转录本中的一部分在 zfs1Δ 突变体中衰减得更慢,并在共免疫沉淀测定中直接与 Zfs1p 结合。一个明显的直接靶标编码转录因子 Cbf12p,当过度表达时,已知会增加细胞间粘附和絮凝。zfs1Δ cbf12Δ 双突变体的研究表明,zfs1Δ 突变体中观察到的絮凝增加至少部分是由于 cbf12 mRNA 周转率的直接影响。这些数据表明,Zfs1p 可以直接和间接地调节该物种中参与细胞间粘附的转录本的水平。

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