显花植物自体和异体花粉识别的分子机理研究

显花植物的受精涉及许多识别过程,其中和线个是雌性生殖组织心皮对花粉的识别。自交不亲和性（Self-incompatibility,SI)是一种广泛分布于显花植物的种内生殖障碍。在多数自交不亲和的植物中,SI的遗传控制比较简单,受控于一个由复等位基因构成的单一位点,称为S位点。在以茄科、玄参科和蔷薇科为代表的配子体自交不亲和植物中,S位编码一类核酸酶,即S核酸酶（Fig.1),控制SI在花柱中的表达,但是与花粉自交不亲和性的表达无关。后者可能由与S核酸酶不同的基因控制,这种基因常被称为花粉S基因。它是目前了解显花植物花粉识别生化和分子机理的关键。近来,通过对影响花粉SI表达突变体的前了解 花植物花粉识别生化和分子机理的关键。近来,通过对影响花粉SI表达突变体的分子遗传分析提出了一个花粉S基因产物如何与S核酸酶相互作用完成自体和异体花粉识别过程的模型（Fig.2)。另外,描述了两个在金鱼草中克隆花粉S基因的方法,即S位点选择性的转座子标记和图位克隆。     

基于S-核酸酶的自交不亲和性的分子机制

自交不亲和性是一种广泛存在于显花植物中的种内生殖障碍,可以抑制近亲繁殖而促进异交。其中,以茄科、玄参科和蔷薇科为代表的配子体自交不亲和性是最常见的类型。这类自交不亲和性是由单一的多态性S-位点所控制。目前的研究发现这一位点至少包含两个自交不亲和反应特异性决定因子：花柱中的S-核酸酶和花粉中的SLF（S-Locus F-box）蛋白。该文将主要介绍并讨论基于S-核酸酶的自交不亲和性分子机制的研究进展。     

高等植物自交不亲和性的分子生物学

自交不亲和性是大多数高等植物防止近亲繁殖的一种遗传屏障。它涉及受精时雄配子（花粉）和雌蕊之间的相互作用。目前,已经分离获得了编码控制雌蕊自交不亲和性的Ｓ基因。在孢子体型自交不亲和的芸苔属中,雌蕊Ｓ基因编码Ｓ位点糖蛋白（ＳＬＧ）和Ｓ受体激酶（ＳＲＫ）。它们可能与磷酸化和去磷酸化参与了的某种信号传递有关,最后导致自交花粉生长的抑制。在配子分配体型自交不亲和的茄科中,雌蕊Ｓ位点糖蛋白为一种核糖核酸酶,称为Ｓ－核酸酶（Ｓ－ＲＮａｓｅ）。自交不亲和反应与Ｓ－核酸酶引起的花粉管ＲＮＡ降解有关,并且可能通过花粉管特异性地摄入Ｓ－核酸酶或者花粉管内存在的特异性的核酸酶抑制剂的作用,达到对自交花粉生长的抑制。另外,从配子体型自交不亲和的罂粟中,分离到了与芸台属和茄科不同的雌蕊Ｓ基因,其作用机理可能与Ｃａ＋＋参与的信号传递有关。     

基于S- 核酸酶的自交不亲和性的分子机制

自交不亲和性是一种广泛存在于显花植物中的种内生殖障碍, 可以抑制近亲繁殖而促进异交。其中, 以茄科、玄参科和蔷薇科为代表的配子体自交不亲和性是最常见的类型。这类自交不亲和性是由单一的多态性S-位点所控制。目前的研究发现这一位点至少包含两个自交不亲和反应特异性决定因子: 花柱中的S-核酸酶和花粉中的SLF(S-Locus F-box)蛋白。该文将主要介绍并讨论基于S-核酸酶的自交不亲和性分子机制的研究进展。     

植物花粉S基因及其应用研究进展

自交不亲和性(self-incompatibility)研究是探讨植物遗传机制和植物育种的重要基础.在显花植物中,配子体自交不亲和由花柱S基因S-RNase和花粉S基因两个基因控制,这两个基因都具有较高的多态性和序列多样性的特征.花粉自交不亲和性是由花粉特异表达的F-box基因控制,命名为SFB(S haplotype-specific F-box protein)基因,并认为它就是花粉S基因的首选.就SFB基因的克隆、结构特点和作用机理以及应用予以综述.     

高等植物自交不亲和性的分子生物学

自交不亲和性是大多数高等植物防止近亲繁殖的一种遗传屏障。它涉及受精时雄配子（花粉）和雌蕊之间的相互作用。目前,已经分离获得了编码控制雌蕊自交不亲和性的Ｓ基因。在孢子体型自交不亲和的芸苔属中,雌蕊Ｓ基因编码Ｓ位点糖蛋白（ＳＬＧ）和Ｓ受体激酶（ＳＲＫ）。它们可能与磷酸化和去磷酸化参与了的某种信号传递有关,最后导致自交花粉生长的抑制。在配子分配体型自交不亲和的茄科中,雌蕊Ｓ位点糖蛋白为一种核糖核酸酶,称     

植物自交不亲和基因研究进展

自交不亲和性的研究是植物生殖生物学和分子生物学研究的热点之一,对自交不亲和基因和蛋白质的深入研究是解析自交不亲和性机理的关键.对控制孢子体自交不亲和性和配子体自交不亲和性的S基因及其蛋白质产物的分子生物学研究进展进行了综述.孢子体自交不亲和性植物S位点上至少存在3个基因,即SLG、SRK和SCR基因.其中SLG、SRK基因控制雌蕊自交不亲和性,而SCR控制花粉自交不亲和性.配子体自交不亲和植物雌蕊S基因产物为S-RNase,具有核酸酶活性;配子体自交不亲和植物花粉S基因产物尚未找到.     

芸苔属植物自交不亲和性的分子机制

芸薹属植物自交不亲和性受单一位点的复等位基因控制,此位点命名为S位点。它决定柱头表面花粉识别的专一性。S位点糖蛋白基因（SLG）和S受体激酶基因（SRK）是控制芸薹属植物花柱自交不亲和性的两个关键因子。本文介绍了编码自交不亲和性的S位点的SLG、SRK和花粉S基因的鉴定、结构及功能,并对其信号传导途径的可能机制做了简要概述。     

自交不亲和植物S—位点特异性糖蛋白

自交不亲和植物Ｓ┐位点特异性糖蛋白朱利泉王晓佳（西南农业大学,重庆６３０７１６）关键词植物自交不亲和性Ｓ－位点特异性糖蛋白多态性植物自交不亲和性是指植物正常的雌雄配子之间花期自交不结实或结实率很低的现象,它在遗传上受Ｓ－位点（Ｓ－ｌｏｃｕｓ）控制。Ｓ...     

芸薹属植物自交不亲和性的分子机制

芸薹属植物自交不亲和性受单一位点的复等位基因控制,此位点命名为S位点,它决定柱头表面花粉识别的专一性,S位点糖蛋白基因（SLG）和S受体激酶基因（SRK)是控制芸薹属植物花柱自交不亲和性的两个关键因子,本文介绍了编码自产不亲和性的S位点的SLG,SRK和花粉S基因的鉴定,结构及功能,并对其信号传导途径的可能机制做了简要概述。     

An F-box gene linked to the self-incompatibility (S) locus of Antirrhinum is expressed specifically in pollen and tapetum

In many flowering plants, self-fertilization is prevented by an intraspecific reproductive barrier known as self-incompatibility (SI), that, in most cases, is controlled by a single multiallelic S locus. So far, the only known S locus product in self-incompatible species from the Solanaceae, Scrophulariaceae and Rosaceae is a class of ribonucleases called S RNases. Molecular and transgenic analyses have shown that S RNases are responsible for pollen rejection by the pistil but have no role in pollen expression of SI, which appears to be mediated by a gene called the pollen self-incompatibility or Sp gene. To identify possible candidates for this gene, we investigated the genomic structure of the S locus in Antirrhinum, a member of the Scrophulariaceae. A novel F-box gene, AhSLF-S2, encoded by the S2 allele, with the expected features of the Sp gene was identified. AhSLF-S2 is located 9 kb downstream of S2 RNase gene and encodes a polypeptide of 376 amino acids with a conserved F-box domain in its amino-terminal part. Hypothetical genes homologous to AhSLF-S2 are apparent in the sequenced genomic DNA of Arabidopsis and rice. Together, they define a large gene family, named SLF (S locus F-box) family. AhSLF-S2 is highly polymorphic and is specifically expressed in tapetum, microspores and pollen grains in an allele-specific manner. The possibility that Sp encodes an F-box protein and the implications of this for the operation of self-incompatibility are discussed.     

Ubiquitin–proteasome‐mediated degradation of S‐RNase in a solanaceous cross‐compatibility reaction

Many plants have a self‐incompatibility (SI) system in which the rejection of self‐pollen is determined by multiple haplotypes at a single locus, termed S. In the Solanaceae, each haplotype encodes a single ribonuclease (S‐RNase) and multiple S‐locus F‐box proteins (SLFs), which function as the pistil and pollen SI determinants, respectively. S‐RNase is cytotoxic to self‐pollen, whereas SLFs are thought to collaboratively recognize non‐self S‐RNases in cross‐pollen and detoxify them via the ubiquitination pathway. However, the actual mechanism of detoxification remains unknown. Here we isolate the components of a SCF^SLF (SCF = SKP1‐CUL1‐F‐box‐RBX1) from Petunia pollen. The SCF^SLF polyubiquitinates a subset of non‐self S‐RNases in vitro. The polyubiquitinated S‐RNases are degraded in the pollen extract, which is attenuated by a proteasome inhibitor. Our findings suggest that multiple SCF^SLF complexes in cross‐pollen polyubiquitinate non‐self S‐RNases, resulting in their degradation by the proteasome.     

Electrostatic potentials of the S‐locus F‐box proteins contribute to the pollen S specificity in self‐incompatibility in Petunia hybrida

Self‐incompatibility (SI) is a self/non‐self discrimination system found widely in angiosperms and, in many species, is controlled by a single polymorphic S‐locus. In the Solanaceae, Rosaceae and Plantaginaceae, the S‐locus encodes a single S‐RNase and a cluster of S‐locus F‐box (SLF) proteins to control the pistil and pollen expression of SI, respectively. Previous studies have shown that their cytosolic interactions determine their recognition specificity, but the physical force between their interactions remains unclear. In this study, we show that the electrostatic potentials of SLF contribute to the pollen S specificity through a physical mechanism of ‘like charges repel and unlike charges attract’ between SLFs and S‐RNases in Petunia hybrida. Strikingly, the alteration of a single C‐terminal amino acid of SLF reversed its surface electrostatic potentials and subsequently the pollen S specificity. Collectively, our results reveal that the electrostatic potentials act as a major physical force between cytosolic SLFs and S‐RNases, providing a mechanistic insight into the self/non‐self discrimination between cytosolic proteins in angiosperms.     

The Skp1‐like protein SSK1 is required for cross‐pollen compatibility in S‐RNase‐based self‐incompatibility

The self‐incompatibility (SI) response occurs widely in flowering plants as a means of preventing self‐fertilization. In these self/non‐self discrimination systems, plant pistils reject self or genetically related pollen. In the Solanaceae, Plantaginaceae and Rosaceae, pistil‐secreted S‐RNases enter the pollen tube and function as cytotoxins to specifically arrest self‐pollen tube growth. Recent studies have revealed that the S‐locus F‐box (SLF) protein controls the pollen expression of SI in these families. However, the precise role of SLF remains largely unknown. Here we report that PhSSK1 (Petunia hybrida SLF‐interacting Skp1‐like1), an equivalent of AhSSK1 of Antirrhinum hispanicum, is expressed specifically in pollen and acts as an adaptor in an SCF(Skp1‐Cullin1‐F‐box)^SLF complex, indicating that this pollen‐specific SSK1‐SLF interaction occurs in both Petunia and Antirrhinum, two species from the Solanaceae and Plantaginaceae, respectively. Substantial reduction of PhSSK1 in pollen reduced cross‐pollen compatibility (CPC) in the S‐RNase‐based SI response, suggesting that the pollen S determinant contributes to inhibiting rather than protecting the S‐RNase activity, at least in solanaceous plants. Furthermore, our results provide an example that a specific Skp1‐like protein other than the known conserved ones can be recruited into a canonical SCF complex as an adaptor.     

A Rewarding Fifteen Years: From SLG to SCR/SP11

Selfincompatibility (SI) is a major genetic mechanism to prevent selffertilization in flowering plants and, in most cases, controlled by a single multiallelic locus, known as the S locus. In Brassica, the genes mediating both stylar (SRK, S receptor kinase) and pollen (SCR/SP11, S locus cystein rich protein/S locus protein 11) expression of selfincompatible reaction have been characterized though the first S locus-encoded gene, SLG (S locus glycoprotein), was isolated nearly fifteen years ago. These findings have finally unveiled the molecular partners in pollen recognition during selfincompatible reaction in Brassica.     

值得的十五年——从SLG到SCR/SP11

Self_incompatibility (SI) is a major genetic mechanism to prevent self_fertilization in flowering plants and, in most cases, controlled by a single multiallelic locus, known as the S locus. In Brassica, the genes mediating both stylar (SRK, S receptor kinase) and pollen (SCR/SP11, S locus cystein rich protein/S locus protein 11) expression of self_incompatible reaction have been characterized though the first S locus_encoded gene, SLG (S locus glycoprotein), was isolated nearly fifteen years ago. These findings have finally unveiled the molecular partners in pollen recognition during self_incompatible reaction in Brassica.     

An F-box gene linked to the self-incompatibility (S) locus of Antirrhinum is expressed specifically in pollen and tapetum

In many flowering plants, self-fertilization is prevented by an intraspecific reproductive barrier known as self-incompatibility (SI), that, in most cases, is controlled by a single multiallelic S locus. So far, the only known S locus product in self-incompatible species from the Solanaceae, Scrophulariaceae and Rosaceae is a class of ribonucleases called S RNases. Molecular and transgenic analyses have shown that S RNases are responsible for pollen rejection by the pistil but have no role in pollen expression of SI, which appears to be mediated by a gene called the pollen self-incompatibility or Sp gene. To identify possible candidates for this gene, we investigated the genomic structure of the S locus in Antirrhinum, a member of the Scrophulariaceae. A novel F-box gene, AhSLF-S ₂, encoded by the S ₂ allele, with the expected features of the Sp gene was identified. AhSLF-S ₂ is located 9 kb downstream of S ₂ RNase gene and encodes a polypeptide of 376 amino acids with a conserved F-box domain in its amino-terminal part. Hypothetical genes homologous to AhSLF-S ₂ are apparent in the sequenced genomic DNA of Arabidopsis and rice. Together, they define a large gene family, named SLF (S locus F-box) family. AhSLF-S ₂ is highly polymorphic and is specifically expressed in tapetum, microspores and pollen grains in an allele-specific manner. The possibility that Sp encodes an F-box protein and the implications of this for the operation of self-incompatibility are discussed.     

Heterochromatic and genetic features are consistent with recombination suppression of the self-incompatibility locus in Antirrhinum

Self-incompatibility (SI) is a genetic mechanism to prevent self-fertilization that is found in many species of flowering plants. Molecular studies have demonstrated that the S-RNase and SLF/SFB genes encoded by the single polymorphic S locus, which control the pollen and pistil functions of SI in three distantly related families, the Solanaceae, Scrophulariaceae and Rosaceae, are organized in a haplotype-specific manner. Previous work suggested that the haplotype structure of the two genes is probably maintained by recombination suppression at the S locus. To examine features associated with this suppression, we first mapped the S locus of Antirrhinum hispanicum, a member of the Scrophulariaceae, to a highly heterochromatic region close to the distal end of the short arm of chromosome 8. Both leptotene chromosome and DNA fiber fluorescence in situ hybridization analyses showed an obvious haplotype specificity of the Antirrhinum S locus that is consistent with its haplotype structure. A chromosome inversion was also detected around this region between A. majus and A. hispanicum. These results revealed that DNA sequence polymorphism and a heterochromatic location are associated with the S locus. Possible roles of these features in maintenance of the haplotype specificity involved in both self and non-self recognition are discussed.     

Pollen S–locus F–box proteins of Petunia involved in S–RNase‐based self‐incompatibility are themselves subject to ubiquitin‐mediated degradation

Many flowering plants show self‐incompatibility, an intra‐specific reproductive barrier by which pistils reject self‐pollen to prevent inbreeding and accept non‐self pollen to promote out‐crossing. In Petunia, the polymorphic S–locus determines self/non‐self recognition. The locus contains a gene encoding an S–RNase, which controls pistil specificity, and multiple S‐locus F‐box (SLF) genes that collectively control pollen specificity. Each SLF is a component of an SCF (Skp1/Cullin/F‐box) complex that is responsible for mediating degradation of non‐self S‐RNase(s), with which the SLF interacts, via the ubiquitin–26S proteasome pathway. A complete set of SLFs is required to detoxify all non‐self S‐RNases to allow cross‐compatible pollination. Here, we show that SLF1 of Petunia inflata is itself subject to degradation via the ubiquitin–26S proteasome pathway, and identify an 18 amino acid sequence in the C‐terminal region of S₂‐SLF1 (SLF1 of S₂ haplotype) that contains a degradation motif. Seven of the 18 amino acids are conserved among all 17 SLF proteins of S₂ haplotype and S₃ haplotype involved in pollen specificity, suggesting that all SLF proteins are probably subject to similar degradation. Deleting the 18 amino acid sequence from S₂‐SLF1 stabilized the protein but abolished its function in self‐incompatibility, suggesting that dynamic cycling of SLF proteins is an integral part of their function in self‐incompatibility.     

Molecular aspects of self-incompatibility in Brassica species.

Many flowering plants possess self-incompatibility (SI) systems to prevent inbreeding. SI in Brassica species is controlled by a single S locus with multiple alleles. In recent years, much progress has been made in determining the male and female S determinant in Brassica species. In the female, a gain-of-function experiment clearly demonstrated that SRK was the sole S determinant, and that SLG enhanced the SI recognition process. By contrast, the male S determinant (termed SP11/SCR) was identified in the course of genome analysis of S locus to be a small cysteine-rich protein, which was classified as a pollen coat protein. This SP11/SCR may function as a ligand for the S domain of SRK in the SI recognition reaction of Brassica species.