配子体自交不亲和植物花粉S基因研究进展

配子体自交不亲和植物的自交不亲和性是由雌蕊自交不亲和因子和花粉自交不亲和因子相互作用的结果。目前已经分离和鉴定了雌蕊自交不亲和基因及其表达产物。最近从金鱼草、Prumusdulcis、梅等植物中分离的F-box基因,它具有花粉S基因特点,即在花药、成熟的花粉和花粉管中特异表达;在基因位置上,与S-RNase基因紧密连锁;不同物种或同一物种不同品种F-box基因间核苷酸和氨基酸序列上存在高度多态性。通过分子生物学方法和杂交授粉试验证明所分离的F-box基因是花粉自交不亲和基因,但目前尚未分离出该类基因相应的表达蛋白。主要综述了配子体自交不亲和植物花粉自交不亲和基因的发现、基因的结构、雌蕊自交不亲和因子和花粉自交不亲和因子相互作用的模型。     

樱桃品种S基因型及自交不亲和性分子机制研究进展

系统介绍了樱桃S基因型鉴定的主要方法,全面列出上百个已知甜樱桃品种的S基因型,其中共涉及16个S基因;着重讨论了樱桃S基因座内S-RNase和SFB基因的研究概况、结构特点及位置关系,并提出该领域善待解决的问题。     

芸苔属植物S受体蛋白激酶的研究

植物的发育过程中信号传导离不开接受信号的受体。受体是靶细胞接受信号或对其作出初步反应的一些特殊蛋白质。主要是细胞表面受体 ,是一类跨膜蛋白质 ,根据其结构和作用方式可分为三大类 :离子通道关联受体、Ｇ蛋白关联受体、酶联受体。酶联受体蛋白本身就是一种酶与酶相联系 ,通常是蛋白质激酶 ,可以使细胞内一些蛋白质磷酸化。在植物自交不亲和 (Ｓｅｌｆ-ｉｎｃｏｍｐａｔｉｂｉｌｉｔｙ ,ＳＩ)反应中 ,有一种重要参与物质 ,称为Ｓ受体蛋白激酶 (Ｓｒｅｃｅｐｔｏｒｋｉｎａｓｅ,ＳＲＫ)就属于酶联受体。自交不亲和现象在芸苔属 (Ｂｒａ…     

24份甜樱桃材料自交不亲和S基因型鉴定

甜樱桃品种绝大部分自交不亲和,限制了甜樱桃的正确评价和合理利用,因此自交不亲和基因型的鉴定对于生产具有重要意义。以24个甜樱桃主栽品种为材料,用5对蔷薇科李属引物组合对24个甜樱桃品种进行了S等位基因的PCR扩增,克隆S基因的扩增片段,用核酸序列在Gen Bank上搜索,确定了5种S基因的核酸序列和大小。结果表明:Pru C2+Pru C4R引物组合扩增效果最好;在琼脂糖凝胶上位置相同的扩增带其核酸序列相同,是同一种S基因;5种S基因扩增片段的大小分别是S1为800 bp,S3为762 bp,S4为962bp,S5为300 bp,S6为456 bp,S9为650 bp;24个甜樱桃S基因型是红手球、早红宝石为S1S3,拉宾斯S1S4',红宝石S1S6,布鲁克斯S1S9,那翁S3S4,秦林、泰安大紫、先锋、早大果、丽珠、美早、5-106、左滕锦、桑提娜为S3S6,黑珍珠、红灯、萨米脱、秦樱为S3S9,胜利为S5S9,明珠、红蜜、雷尼、滨库为S6S9。     

甜樱桃(Prunus avium L.)品种S基因型鉴定

根据蔷薇科S-RNase基因(S基因)高度保守区C2和RC4区设计一对特异引物PruC2和PruC4R,对甜樱桃品种的基因组DNA进行S基因特异PCR扩增。克隆S基因的扩增片段,核酸序列在GenBank上搜索,确定了4种S基因的核酸序列和大小。结果表明,在琼脂糖凝胶上位置相同的扩增带其核酸序列相同,是同一种S基因。4种S基因扩增片段的大小分别是：S1为677bp,S3为762bp,S4为945bp,S6为456bp。参试的自交不亲和品种的S基因型分别是：红灯、红艳、早红宝石和先锋相同,为S1S3;抉择、红丰和那翁相同,为S3S4;大紫为S1S6;长把红为S1S4;养老为S2S6;自交亲和品种外引7号和斯太拉为S3S4。     

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.     

花粉特异F-box基因及其表达产物可能参与的SCF途径

泛素蛋白体目标性降解蛋白途径是许多细胞学过程的重要调节体系,底物蛋白泛素化涉及3个酶激反应,其中,作为E3连接酶的SCF复合体对底物的识别是通过亚体F-box蛋白C末端的特异性结构实现的.利用染色体步移等方法,最近在一些配子体型自交不亲和植物S-RNase基因近旁相继发现了一类花粉特异性表达的F-box基因,从而预示泛素介导的SCF蛋白降解途径可能参与配子体自交不亲和反应.     

植物孢子体自交不亲和信号转导功能分子研究进展

孢子体自交不亲和(SSI)是许多植物采取的一种抵制近亲繁殖的重要措施,受S位点复等位基因控制。近年来,参与其信号转导的许多功能分子及它们的编码基因被分离并得到了充分研究：当自花授粉时,SPlI／SCR与SRK特异识别,造成后的Ser／Thr激酶的磷酸化,引发了一系列由SLG、ARC1及水孔蛋白等因子参与的SSI信号转导途径,最终产生自交不亲和的结果。     

芸苔属植物自交不亲和性及其机理研究进展

自交不亲和性广泛存在于芸苔属植物当中,有着防止自交衰退等作用,在育种工作中意义重大。本文综述了芸苔属植物自交不亲和性及其表现,自交不亲和内在机制,如S复等位基因及相互作用,S位点糖蛋白,S多基因家族,S位点受体激酶,蛋白质可逆磷酸化等 。     

植物受体蛋白激酶的研究进展

在植物中存在一种由胞外结构域、跨膜区域和胞内的蛋白激酶区域三部分组成的跨膜受体蛋白激酶（receptor-lik protein kinases,RLKs)。该蛋白一方面作为胞外特异配基的受体,同时本身又是一种蛋白激酶。研究表明,植物细胞中的RLKs可能参与了植物细胞抗逆反应,植物形态发生、自交不亲和等生理生化反应,作者将从RLKs的结构、种类,基因表达方式及其植物生长和发育过程中的作用做简要介绍。     

Subcellular Localization of the S Locus F-box Protein AhSLF-S2 in Pollen and Pollen Tubes of Self-Incompatible Antirrhinum

The distribution of the S locus F-box (SLF) protein was examined by immunocytochemistry and Western blot techniques using an antibody against the C-terminal part of AhSLF-S2 in self-incompatible lines of Antirrhinum. Abundant gold particles were found where pollen tubes emerge in vitro. With the elongation of pollen tubes, binding sites for the antibody were found in the cytoplasm of the pollen tubes,including the peripheral part of the endoplasmic reticulum. After germination in vitro for 16 h, the product of AhSLF-S2 and possibly its allelic products could still be detectable, implying that the SLF protein has a role in the elongating process of pollen tubes. The present study provides evidence at the protein level that the SLF protein is present in pollen cytoplasm during pollen tube growth. These findings are discussed, as is their potential role in the self-incompatible response in Antirrhinum.     

Subcellular Localization of the S Locus F-box Protein AhSLF-S2 in Pollen and Pollen Tubes of Self-Incompatible Antirrhinum

The distribution of the S locus F-box (SLF) protein was examined by immunocytochemistry and Western blot techniques using an antibody against the C-terminal part of AhSLF-S2 in self-incompatible Iines of Antirrhinum. Abundant gold particles were found where pollen tubes emerge in vitro. With the elongation of pollen tubes, binding sites for the antibody were found in the cytoplasm of the pollen tubes,including the peripheral part of the endoplasmic reticulum. After germination in vitro for 16 h, the product of AhSLF-S2 and possibly its allelic products could still be detectable, implying that the SLF protein has a role in the elongating process of pollen tubes. The present study provides evidence at the protein level that the SLF protein is present in pollen cytoplasm during pollen tube growth. These findings are discussed, as is their potential role in the self-incompatible response in Antirrhinum.     

The use of the S haplotype-specific F-box protein gene,SFB, as a molecular marker for S-haplotypes and self-compatibility in Japanese apricot (Prunus mume)

Japanese apricot (Prunus mume) exhibits the S-RNase-based gametophytic self-incompatibility system as do other self-incompatible Prunus species. This report identifies the S haplotype-specific F-box protein gene (SFB), a candidate gene for pollen-S, of Japanese apricot, which leads to the development of a molecular typing system for S-haplotype in this fruit species. Both 5- and 3-RACE (rapid amplification of cDNA ends) were performed with SFB gene-specific oligonucleotide primers to clone Pm-SFB¹ and Pm-SFB⁷ of 'Nanko (S¹S⁷)'. As in the case of SFB of other Prunus species, Pm-SFB¹ and Pm-SFB⁷ showed a high level of S-haplotype-specific sequence polymorphism and their expression was specific to pollen. Genomic DNA-blot analyses of 11 Japanese apricot cultivars with the Pm-SFB probes under low stringency conditions yielded RFLP bands specific to the S¹- to S⁸-haplotypes as well as a self-compatible S^f-haplotype. A practical usage of SFB as a molecular marker for S-haplotypes and self-compatibility in Japanese apricot is discussed.Communicated by H.F. LinskensThe nucleotide sequences reported in this paper have been submitted to the EMBL/GenBank/DDBJ database under accession numbers, AB101440 and AB101441, for SFB¹ and SFB⁷, respectively     

Pollen stigma interactions in Brassica oleracea

Summary Recent studies on the mechanism of self-incompatibility in Brassica indicate the location, nature and mode of action of the molecules involved. Characteristics of the pollen surface and the stigma surface are described in detail, together with new information pertaining to the recognition molecules located therein. A sequence of events is outlined leading from pollination, through adhesion, hydration, germination, and tube growth to acceptance and ultimate compatibility. The characteristics of rejection of incompatible grains are described for each stage of the pollen-stigma interaction. It is proposed that recognition of proteins from the coating of self-pollen by the molecules in the pellicle results in the formation of a biologically-active complex which inhibits water supply to the incompatible grain, and that all other manifestations of incompatibility are a consequence of this initial response.     

Agrobacterium-Mediated Transfer of the GUS Gene into Pollen of Petunia

Transfer of the GUS gene into pollen has been studied in co-cultures of Agrobacterium and Petunia pollen. The Agrobacterium strain used contains a GUS gene between the two borders of the T-DNA. Uptake and integration of this GUS gene could be shown using two different restriction systems. First, by appropriate cleavage within the T-DNA the GUS gene could be isolated intact from Agrobacterium-treated pollen. Second, using enzymes with cleave the T-DNA only once, integration of this T-DNA into individual pollen genomes could be shown. The fragments obtained could not be obtained from Agrobacterium alone. The positive Southern blots were reprobed with vir probes, but all were negative. Also following plating, no Agrobacteria could be detected from our pollen DNA preparations. Therefore, the signals obtained were not due to contaminating bacteria. Due to a high endogenous GUS activity of Petunia pollen the expression of the transferred gene could not be studied. The data demonstrate the uptake and integration of T-DNA into pollen and are closing a gap in the line of evidence for the functioning of an indirect Agrobacterium — mediated gene transfer. Besides this, it should be stressed that only this indirect pollen system leads to success.     

外源基因导入技术在主要农作物育种上的应用进展

以国内科技期刊上发表的文献研究结果为依据,综述了农杆菌介导技术、基因枪导入技术、花粉管通道技术与激光微束穿刺技术在小麦、水稻、棉花、大豆、油菜等主要农作物育种上的应用进展。同时,还简要介绍了其中主要外源基因导入技术的基本原理,并评价了其优缺点。     

Plant size,geitonogamy and seed set in Ipomopsis aggregata

Summary We used powdered fluorescent dyes to estimate receipt of self vs. outcross pollen in the self-incompatible species Ipomopsis aggregata (Polemoniaceae). Flowers on small and large plants received equal amounts of outcross pollen, whereas flowers on large plants received more self pollen, so the proportion of self pollen delivered through geitonogamy increased with plant size. In natural populations emasculation of all flowers on a plant raised average seed set per flower from 5.19 to 6.99 and also raised fruit set, though not significantly. From these results one expects a negative correlation between plant size and seeds per flower. The opposite trend was observed in a sample of plants in the field, suggesting that deleterious effects of geitonogamy on female fecundity in large plants can be overruled by other factors such as size-related fruit or seed abortion. Results are discussed in relation to the evolution of gynodioecy.