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国家自然科学基金(30500348)

作品数:4 被引量:27H指数:4
相关作者:张志宏代红艳马跃赵桂玲王昆更多>>
相关机构:沈阳农业大学中国农业科学院果树研究所更多>>
发文基金:国家自然科学基金辽宁省高等学校优秀人才支持计划国家教育部博士点基金更多>>
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Genome-wide Characterization of Long Terminal Repeat-retrotransposons in Apple Reveals the Differences in Heterogeneity and Copy Number between Ty1-copia and Ty3-gypsy Retrotransposons被引量:7
2008年
The conserved domains of reverse transcriptase (RT) genes of Tyl-copia and Ty3-gypsy groups of long terminal repeat (LTR) retrotransposons were isolated from the Malus domestica genome using degenerate oligonucleotide primers. Sequence analysis showed that 45% of Ty1-copia and 63% of Ty3-gypsy RT sequences contained premature stop codons and/or indels disrupting the reading frame. High heterogeneity among RT sequences of both Ty1-copia and Ty3-gypsy group retrotransposons was observed, but Ty3-gypsy group retrotransposons in the apple genome are less heterogeneous than Ty1-copia elements. Retrotransposon copy number was estimated by dot blot hybridizations for Ty1-copia (-5000) and Ty3-gypsy (-26000). All elements of the two types of LTR retrotransposons comprise approximately 38% of the M. domestica genome, with the Ty3-gypsy group contribution being higher (33.5%) than the Tyl.copia one (4.6%). Transcription was not detected by reverse transcription-polymerase chain reaction for either Ty1-copia or Ty3-gypsy retrotransposons in the leaves of plants in vitro or in leaf explants cultured on medium supplemented with high concentration benzylaminopurine. This research reveals the differences in heterogeneity and copy number between Ty1-copia and Ty3-gypsy retrotransposons in the apple genome. Ty1-copia retrotransposon has higher heterogeneity than Ty3-gypsy retrotransposon, but the latter has a higher copy number, which implies that Ty3-gypsy retrotransposons may play a more important role in the apple genome evolution.
Hai-Yue SunHong-Yan DaiGui-Ling ZhaoYue MaChun-Qing OuHe LiLin-Guang LiZhi-Hong Zhang
关键词:HETEROGENEITYRETROTRANSPOSON
苹果S-SAP分子标记体系建立及应用被引量:4
2010年
【目的】建立和优化苹果S-SAP分子标记体系,探讨应用S-SAP技术区分元帅芽变的可能性,为从DNA分子水平上对苹果芽变鉴定和利用奠定基础。【方法】利用富士、寒富和嘎啦初步建立S-SAP分析体系;根据谱带量和多态性等对32对引物组合进行筛选;从DNA酶切、PCR扩增、银染方法等角度对影响S-SAP反应的因子进行优化;利用6对多态性引物,对8个元帅芽变进行S-SAP分析,采用NTsys-pc2软件的SIMQUAL程序计算相似系数,UPGAM方法进行循环同化阶层聚类分析,并通过Treeplot程序生成聚类图。【结果】优化的苹果S-SAP分析体系为,改良CTAB法提取基因组总DNA;MseⅠ和PstⅠ双酶切基因组总DNA;Fermentas公司的TaqDNA聚合酶进行PCR扩增;6%变性聚丙烯酰胺凝胶分离选择性扩增产物;改良弱碱法银染检测差异片段。筛选出6个适宜苹果品种分析的S-SAP引物。发现LTRP1/Mtcc引物组合在元帅芽变分析中具有多态性,矮红、红星与新元帅等具有多态性位点,供试芽变资源的遗传相似系数在0.88—0.98之间,以相似系数0.93为标准,8个元帅芽变资源可分为4类。【结论】建立了基于Ty1-copia组反转录转座子的苹果S-SAP标记体系,筛选出了6个适宜苹果品种分析的S-SAP引物,利用LTRP1/Mtcc引物组合成功区分了元帅芽变。
赵桂玲张志宏马跃常琳琳王昆代红艳
关键词:苹果
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