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番茄野生型和phytochrome A缺陷型突变体中PHYA的分子分析。

Molecular analysis of PHYA in wild-type and phytochrome A-deficient mutants of tomato.

作者信息

Lazarova G I, Kerckhoffs L H, Brandstädter J, Matsui M, Kendrick R E, Cordonnier-Pratt M M, Pratt L H

机构信息

Laboratory for Photoperception and Signal Transduction, Institute of Physical and Chemical Research (RIKEN), Saitama, Japan.

出版信息

Plant J. 1998 Jun;14(6):653-62. doi: 10.1046/j.1365-313x.1998.00164.x.

Abstract

Tomato (Lycopersicon esculentum Mill., recently redesignated Solanum lycopersicum L.), an agronomically important crop plant, has been adopted as a model species complementary to Arabidopsis in which to characterize the phytochrome family. Here we describe the cloning and molecular characterization of the gene encoding the apoprotein of phytochrome A in wild-type tomato and in the far-red-light-insensitive (fri1 and fri2) tomato mutants. The physical organization of this gene is similar to that of other angiosperm phytochromes with the four exons of the coding region interrupted by three introns. The pool of transcripts is heterogeneous due to multiple transcription start sites and to three modes of alternative splicing of the 5' leader. The leader in each alternative transcript carries multiple upstream open reading frames of considerable length. At the genomic level, both fri mutants share an identical base substitution which changes a consensus AG/ to TG/ at the 3' end of the intron between exons 1 and 2. This mutation leads to aberrant processing of the resultant pre-mRNA. While most mature transcripts retain the mutated intron, both cryptic splicing and exon skipping were also detected. Cryptic splicing occurred both upstream and downstream from the wild-type splice site. These observations are consistent with the hypothesis that exon definition in splicing of plant pre-mRNAs plays a secondary role to that of intron definition. Analysis of the frequency with which potentially functional phytochrome A apoproteins might be produced indicates that both fri1 and fri2 have less than 1% of the wild-type phytochrome A level.

摘要

番茄(Lycopersicon esculentum Mill.,最近重新命名为Solanum lycopersicum L.)是一种在农业上具有重要意义的作物,已被用作与拟南芥互补的模式物种,用于对植物光敏色素家族进行特性描述。在此,我们描述了野生型番茄和远红光不敏感(fri1和fri2)番茄突变体中编码光敏色素A脱辅基蛋白基因的克隆及分子特性。该基因的物理结构与其他被子植物光敏色素相似,编码区的四个外显子被三个内含子隔开。由于多个转录起始位点以及5'前导序列的三种可变剪接模式,转录本群体具有异质性。每个可变转录本中的前导序列都带有多个长度可观的上游开放阅读框。在基因组水平上,两个fri突变体都存在相同的碱基替换,该替换将外显子1和2之间内含子3'端的共有AG/变为TG/。这种突变导致产生的前体mRNA加工异常。虽然大多数成熟转录本保留了突变的内含子,但也检测到了隐蔽剪接和外显子跳跃。隐蔽剪接发生在野生型剪接位点的上游和下游。这些观察结果与以下假设一致,即植物前体mRNA剪接中的外显子定义相对于内含子定义起次要作用。对可能产生有功能的光敏色素A脱辅基蛋白的频率分析表明,fri1和fri2的光敏色素A水平均不到野生型的1%。

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