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Pollen dispersal was estimated in two test plots in a hinoki (Chamaecyparis obtusa) seed orchard using a chloroplast DNA marker, the spacer region between thetrnD andtrnY genes, and SSCP (single strand conformation polymorphism). In Plot 1, 2,020 seeds from 40 trees within 30 m of the marker
tree were analyzed using the PCR-SSCP method. In Plot 2, 1,850 seeds from 37 trees were analyzed in the same manner. The results
revealed that the maximum pollen dispersal distance in the two plots exceeded 25 m. Pollen dispersal appeared to be inversely
proportional to the distance from the marker tree. The effective pollen dispersal was suggested to be less than about 20 m
in a mature hinoki seed orchard. Adjacent trees had an excessive influence when the pollen density was increased by artificial
flower stimulation. Therefore, it was suggested that seed production better resembles ideal random mating when carried out
as naturally as possible. In conclusion, the SSCP chloroplast DNA marker was a useful tool for amassing basic information
on pollen management in seed orchards of coniferous species. 相似文献
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G. Yang R. Forrest H. Zhou S. Hodge J. Hickford 《Zeitschrift für Tierzüchtung und Züchtungsbiologie》2014,131(6):437-444
The uncoupling protein 1 (UCP1) plays an important role in the regulation of lipolysis and thermogenesis in adipose tissues. Genetic variation within three regions (the promoter, intron 2 and exon 5) of the ovine UCP1 gene (UCP1) was investigated using polymerase chain reaction‐single‐strand conformational polymorphism (PCR‐SSCP) analyses. These revealed three promoter variants (designated A, B and C) and two intron 2 variants (a and b). The association of this genetic variation with variation in lamb carcass traits and postweaning growth was investigated in New Zealand (NZ) Romney and Suffolk sheep. The presence of B in a lamb's genotype was associated with decreased subcutaneous carcass fat depth (V‐GR) (p = 0.004) and proportion of total lean meat yield of loin meat (p = 0.005), and an increased proportion of total lean meat yield of hind‐leg meat (p = 0.018). In contrast, having two copies of C was associated with increased V‐GR (p < 0.001) and proportion of total lean meat yield of shoulder meat (p = 0.009), and a decreased hind‐leg yield (p = 0.032). No associations were found with postweaning growth. These results suggest that ovine UCP1 is a potential gene marker for carcass traits. 相似文献
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This study describes variation of intron-3 of a-amylase gene from 156 breeds of adzuki beansusing SSCP(single-strand conformation polymorphism)analysis. Based on a-amylase gene structure and se-quence, A pair of PCR primers, F (CCTACATTCTAACACACCCT) and R (GCATATTGTGCCAGTACAAT)were designed to amplify intron-3 fragments of a-amylase gene. 14 variant types were detected, including 13,9, 10, 4 variant types in the wild, weed, locally cultivated and modern brought-up adzuki beans respectively,9, 8, 7 variant types of the wild adzuki beans from Japan, China and Korea respectively, and some other va-riant types in the local adzuki beans from China and Bhutan. 60 % of subjects of cultivated races were found tobe EE type in the experiment. In addition, sequence analysis of intron-3 of α-amylase gene from 8 varianttypes reveals the evolution process of various variant types in adzuki beans. 相似文献
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重庆地区柑桔衰退病毒组群分析 总被引:4,自引:1,他引:4
柑桔衰退病毒(CTV)存在着许多生物学特性不同的株系。通过铲除感染强毒株植株或利用弱毒株交叉保护的方式来防治柑桔衰退病都需要对CTV株系进行准确、可靠的鉴定。根据对CTV衣壳蛋白基因(CPGs)的限制性片段长度多态性(RFLP)和单链构象多态性(SSCP)分析,发现在重庆地区CTV主要以CP/HinfⅠRFLP第1,3和6组群为主,并且在田间以多株系混合感染为主? 相似文献
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PLIN基因多态性及其与绵羊尾形和屠宰性状的关联研究 总被引:1,自引:0,他引:1
为了探讨PLIN基因多态性及其对绵羊经济性状的影响,利用PCR-SSCP技术对2个绵羊品种96个个体PLIN基因的9个外显子进行多态性分析,并将检测到的不同基因型与尾形和屠宰性状进行关联分析。结果表明:外显子3、4、5、6和8存在多态。外显子4的BB型个体的相对尾脂重显著大于AA和AB型个体(P<0.05);外显子6的AA型个体的相对尾脂重显著大于AB和BB型个体(P<0.05);外显子5的不同基因型个体间尾宽差异极显著(P<0.01),且AA型个体的尾宽大于AB型个体。PLIN基因的多态性对绵羊脂肪沉积有一定影响,可作为影响肉质性状的候选基因,从分子水平上指导肉用绵羊的育种工作。 相似文献
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五指山猪近交系群体中DRA和DRB基因的SSCP检测 总被引:10,自引:0,他引:10
为确定五指山猪(WZSP)近交系群体SLA!ⅡDRA、DRB基因的等位基因数及其特性,利用PCR扩增SLA!ⅡDRA、DRB基因的第2外显子序列,经单链构象多态性即SSCP检测其等位基因数,选择纯合子个体的PCR产物直接测序。对所获得的序列与Genbank中所有相应的序列进行比对和聚类分析,特别是SLA!DRB!C、SLA!DRB!D、HLA!DRB*09012、HLA!DRB*1201、HLA!DRA*0101等位基因。结果表明:在WZSP近交系群体中,DRA、DRB各有2个等位基因且发现1个DRB新等位基因。DRA第2外显子有很强的保守性,而DRB基因呈现出高度的多态性,在核苷酸水平同源性为85%以上,氨基酸水平同源性为70%以上。该试验成功地检测了WZSP近交系SLA!DRA、DRB基因的等位基因及其特性,为建立WZSPSLA!DR基因抗原的分子分型及特异单倍型猪的培育研究奠定基础。 相似文献
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SSCP Marker Development and Analysis of Candidate Restorer Gene Rf1 for Cotton Cytoplasmic Male Sterility 总被引:1,自引:0,他引:1
Liu Licai Guo Liping Qi Tingxiang Wang Hailin Tang Huini Zhang Xuexian Qiao Xiuqin Wu Jianyong Xing Chaozhu 《棉花学报》2018,30(1):12-20
[Objective] Locating the cotton cytoplasmic male sterility (CMS) restorer gene Rf1 is important for investigating restorer gene mechanisms and improving restorer lines. In our previous study, a gene cluster, with nine Pentatricopeptide repeat(PPR) genes and nine other genes, was found within the 160-kb Rf1 target region in Scaffold 333. The objective here was to improve the density of Rf1-linked markers in the target region and determine the expression profiles of candidate genes. [Method] Using the sequences of the 18 genes, we designed 155 single-strand conformation polymorphism (SSCP) primers covering all of the gene sequences to identify the polymorphic SSCP markers between the fertile and sterile pools. Additionally, real-time polymerase chain reaction(PCR) was performed to analyze the expression profiles of eight candidate genes in the four developmental stages of buds of sterile, maintainer and restoring lines, respectively. [Result] In total, 15 polymorphic primers were identified. A genotype analysis of the F2 population was conducted using the 15 primers and 3 other polymorphic simple sequence repeats (SSR) markers. The markers were distributed in a 4.8 cM range. In addition, owing to the influence of sterile cytoplasm or restorer genes, most of the genes showed different expression patterns in the four developmental stages of the three lines' buds. [Conclusion] SSCP markers tightly linked to Rf1 were identified and the expression profiles of candidate genes were determined. This study provides a basis for the further fine mapping of restorer genes and for candidate gene screening. 相似文献
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Several SNP (single nucleotide polymorphism) genotyping methods have been developed in the past most of which require sophisticated instrumentation and large initial investments. We describe here a high-throughput SSCP (single strand conformation polymorphism) system on our HEGS (high efficiency genome scanning) platform, which is simple, accurate, cost effective and requires neither restriction digestion of the amplification products nor elaborate post-PCR processing detection. Several parameters critical to SSCP analysis were optimized viz., gel matrix and concentration, gel running temperature, buffer composition, running conditions and PCR primer design so as to identify SNPs in amplicons ranging from 100 to 750 bp in size. A simple post-PCR processing system was developed using fluorescent dye for quick and easy detection of SNP polymorphism. HEGS-SSCP was also found to be useful in uncovering simple sequence repeat differences between different genotypes that differ by one or few di/tri nucleotide repeats. The practical utility of this system is illustrated with two successful efforts towards construction of high resolution linkage maps of a lesion mimic locus on chromosome 7 and a major quantitative trait locus conditioning field blast resistance on chromosome 4 in rice. 相似文献