棉属海岛棉×拟似棉F_1不育性研究

本文研究了棉属海岛棉［ＧｏｓｓｙｐｉｕｍｂａｒｂａｄｅｎｓｅＬ．，（ＡＤ）２］ｘ拟似棉［Ｇ．ｇｏｓｓｙｐｉｏｉｄｅｓ（Ｕ１ｂｒ）Ｓｔａｎｄｌｅｙ，Ｄ６］Ｆ_１植株的减数分裂及不育花粉的形成过程。Ｆ_１花粉母细胞在减数分裂中期Ｉ平均染色体构型为２４．８６Ⅰ＋６．９８Ⅱ＋０．０５Ⅲ。Ｆ_１不育的根本原因在于减数分裂中期染色体不能正常配对，引起部分染色体滞后及染色体不均等分配，从而产生多分孢子和微核，最终导致不育花粉的产生，并讨论Ｄ６与（ＡＤ）２间的亲缘关系以及克服Ｆ_１不育的方法。

粳稻品种4502与广亲和品种间杂种F_1不育性的遗传分析

利用9个籼、粳稻品种,7个广亲和品种,配制单交F_1、回交及三交组合,研究了粳稻品种4502与广亲和品种间F_1不育性的遗传。根据与品种4502杂交F_1的亲和性,可将参试的广亲和品种分为两组,Ⅰ组是与4502亲和的品种,如Dular和02428;Ⅱ组是与4502不亲和的品种,如热研1号、Moroberekan和CPSLO 17。回交和三交组合的育性分离表明,4502和Ⅱ组广亲和品种间杂种F_1花粉不育性受单座位孢子体—配子体等位基因互作控制,将这一基因座暂定名为S-D(t)。广亲和品种Dular在此基因座具有广亲和基因S^n-D(t)。

水稻F1花粉不育基因S-e的初步鉴定

选用分布于水稻12条染色体上74个多态性SSR标记，对E47—1／广陆矮4号的F2分离群体进行偏态分离分析．结果表明，9个SSR标记的分离显著或极显著地偏离了预期的孟德尔比例（1：2：1）．其中，7个SSR标记基因型偏向于籼型，2个标记偏向杂合型，没有发现偏向粳型的标记．通过对第6和第12染色体上4个SSR标记基因型与F2植株花粉育性的初步分析，表明位于第12染色体上SSR标记RM19～RM453区域附近存在1个F，花粉不育基因，定名为S-e．这一结果为分子定位该基因奠定了基础．

Mapping of S-b Locus for F_1 Pollen Sterility in Cultivated Rice Using PCR Based Markers

In cultivated rice ( Oryza sativa L.), F-1 pollen sterility is controlled by at least 6 loci of the F, pollen sterility genes. To map S-b, one of loci, rice variety Taichung 65 (T65) carrying S-b(j)/S-b(j) and its near-isogenic line TIST2 carrying S-b(i)/S-b(i) were used to develop the mapping population. One hundred and fifty-eight microsatellite markers were selected to survey T65 and TISL2. RM13 on chromosome 5 was found to be polymorphic between them. Cosegregation indicated that RM13 was closely linked with locus S-b. Eleven RFLP markers were selected on the corresponding region from the genetic map of Rice Genome Research Program (RGP) of Japan to convert into sequence-tagged site (STS) markers. Amplicon length polymorphism (ALP) was carried out, but none of them was found to be polymorphic between T65 and TISL2. Then PCR-based RFLP (PBR) was done using six 4-nucleotide recognizing restriction endonucleases. Polymorphism was detected when PCR products of R830STS and R2213SSTS were digested with Taq I. Genetic analysis indicated that the distance between locus S-b and markers, R830STS, RM13 and R2213SSTS were 3.3 cM (centi-Morgan), 5.2 cM and 5.5 cM, respectively. These PCR-based markers could be directly used in marker-assisted selection. The technical system combining genetic mapping and PCR-based marker-assisted selection will facilitate the development of molecular breeding.

从普通野生稻中鉴定栽培稻F_1花粉不育座位Sb的中性基因

花粉不育是栽培稻(Oryza sativa L.)籼粳亚种间杂种F1普遍存在的现象,是杂种优势利用的主要障碍之一.至少有6个基因座位控制籼粳亚种间F1的花粉不育,各座位存在的花粉育性中性基因可望克服各自的不育性,所以挖掘和利用不同座位的花粉育性中性基因具有重要意义.本文在栽培稻F1花粉不育基因Sb座位已精细定位和广东高州普通野生稻(O.rufipogen Griff.)(以下简称高州野生稻)具有丰富遗传多样性的基础上,分别以粳稻台中65(编号为E1,基因型SbjSbj)及其Sb座位的近等基因系E2(基因型SbiSbi)为母本,12份不同编号的高州野生稻分别为父本,组配成对测交组合并检测各组合F1的花粉育性,初步鉴定可能具有花粉育性中性基因的材料,并发展相应的F2群体,利用4对与Sb座位紧密连锁的分子标记,分析上述成对测交组合F2群体分子标记的分离情况,并与花粉育性的分离进行统计检验.结果表明,编号为GZW099的高州野生稻与E1及E2组配的成对测交组合的F1花粉育性分别为(89.22±1.07)%和(85.65±1.05)%,表现正常可育且经t检验差异不显著;4对分子标记在相应的F2群体中的3种基因型分离比例符合孟德尔分离比例(1:2:1),且3种基因型对应的平均花粉育性差异不显著,说明该编号的野生稻在Sb座位携带的等位基因与台中65及E2的等位基因均不存在显著互作,因此鉴定GZW099在Sb座位携带花粉育性中性基因,命名为SbnSbn,为进一步研究和克服籼粳杂种不育性提供了理论基础和遗传资源.