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扁桃(Prunus dulcis)S-RNase等位基因分析:新序列特征、同义序列解析及基因内重组证据

Analysis of S-RNase alleles of almond (Prunus dulcis): characterization of new sequences, resolution of synonyms and evidence of intragenic recombination.

作者信息

Ortega Encarnación, Bosković Radovan I, Sargent Daniel J, Tobutt Kenneth R

机构信息

East Malling Research, New Road, East Malling, Kent, ME19 6BJ, UK.

出版信息

Mol Genet Genomics. 2006 Nov;276(5):413-26. doi: 10.1007/s00438-006-0146-4. Epub 2006 Aug 22.

Abstract

Cross-compatibility relationships in almond are controlled by a gametophytically expressed incompatibility system partly mediated by stylar RNases, of which 29 have been reported. To resolve possible synonyms and to provide data for phylogenetic analysis, 21 almond S-RNase alleles were cloned and sequenced from SP (signal peptide region) or C1 (first conserved region) to C5, except for the S29 allele, which could be cloned only from SP to C1. Nineteen sequences (S4, S6, S11-S22, S25-S29)) were potentially new whereas S10 and S24 had previously been published but with different labels. The sequences for S16 and S17 were identical to that for S1, published previously; likewise, S15 was identical to S5. In addition, S4 and S20 were identical, as were S13 and S19. A revised version of the standard table of almond incompatibility genotypes is presented. Several alleles had AT or GA tandem repeats in their introns. Sequences of the 23 distinct newly cloned or already published alleles were aligned. Sliding windows analysis of Ka/Ks identified regions where positive selection may operate; in contrast to the Maloideae, most of the region from the beginning of C3 to the beginning of RC4 appeared not to be under positive selection. Phylogenetic analysis indicated four pairs of alleles had "bootstrap" support > 80%: S5/S10, S4/S8, S11/S24, and S3/S6. Various motifs up to 19 residues long occurred in at least two alleles, and their distributions were consistent with intragenic recombination, as were separate phylogenetic analyses of the 5' and 3' sections. Sequence comparison of phylogenetically related alleles indicated the significance of the region between RC4 and C5 in defining specificity.

摘要

扁桃中的交叉亲和性关系由一个配子体表达的不亲和系统控制,该系统部分由花柱核糖核酸酶介导,已报道了29种花柱核糖核酸酶。为了解决可能存在的同义词问题并为系统发育分析提供数据,从信号肽区域(SP)或第一个保守区域(C1)到C5克隆并测序了21个扁桃S - 核糖核酸酶等位基因,但S29等位基因只能从SP克隆到C1。19个序列(S4、S6、S11 - S22、S25 - S29)可能是新的,而S10和S24此前已发表,但标签不同。S16和S17的序列与之前发表的S1相同;同样,S15与S5相同。此外,S4和S20相同,S13和S19也相同。给出了扁桃不亲和基因型标准表的修订版。几个等位基因在其内含子中有AT或GA串联重复。对23个不同的新克隆或已发表的等位基因序列进行了比对。Ka/Ks的滑动窗口分析确定了可能存在正选择的区域;与苹果亚科不同,从C3开始到RC4开始的大部分区域似乎没有受到正选择。系统发育分析表明,四对等位基因具有“自展”支持率> 80%:S5/S10、S4/S8、S11/S24和S3/S6。至少在两个等位基因中出现了长达19个残基的各种基序,它们的分布与基因内重组一致,5'和3'部分的单独系统发育分析也是如此。系统发育相关等位基因的序列比较表明,RC4和C5之间的区域在定义特异性方面具有重要意义。

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