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1.
南疆沙蜥Phrynocephalus forsythii是我国特有的一种小型爬行动物,分布于塔里木盆地。利用Roche 454 GS FLX高通量测序对该物种基因组测序,获得了55 909条高质量序列。利用Krait搜索并初步统计和分析基因组微卫星序列,共得到1~6个碱基重复类型的完美型微卫星12 109个。不同类型微卫星中,四碱基重复类型数目最多,有4 037个,约占总数的33.34%,其次是二碱基,约占总数的28.09%,再是三碱基、单碱基、五碱基和六碱基,分别约占总数的18.72%、13.91%、4.48%和1.46%。单碱基微卫星中C最多,二碱基微卫星中AC最多,三碱基、四碱基、五碱基和六碱基中最多的分别是AAC、AAAT、AAAAT和AACCCT。AC、AAAT、C、AG、A、AAC、AAT、AAAC、ACC和ACG是数量最多的10种重复拷贝类别。挑选部分三、四碱基重复类型的微卫星序列设计了100对可用于后续对南疆沙蜥微卫星标记开发的候选引物。本研究开启了对南疆沙蜥基因组微卫星特征的了解,为利用微卫星标记研究南疆沙蜥种群遗传结构奠定了基础。  相似文献   

2.
旨在为大规模开发诸氏鲻虾虎鱼微卫星标记,采用高通量测序技术,对诸氏鲻虾虎鱼肝脏转录组进行了测序。结果共获得47 979条Unigenes,利用微卫星查找程序在47 979条Unigenes中共获得6 225个微卫星位点(12.97%),平均每7.02 kb就出现1个微卫星位点。6 225个微卫星位点由226种重复基序组成,主要分布在三、四和五碱基重复类型中。在数量上,单碱基重复类型微卫星位点最多,占42.49%,二碱基和三碱基重复类型所占比例相似,分别为25.22%和26.27%,四、五、六重复类型较少,合计占6.03%。单碱基重复序列中最多的类型为A/T,二碱基重复序列中以AG/CT重复单元为主,三碱基重复序列中以AGC/TCG为优势类型。挑选部分二、三和四单元重复类型微卫星序列,共设计76对引物,可稳定扩增出目的条带的有55对,其中32对具有多态性。结果表明,利用诸氏鲻虾虎鱼转录组数据可快速大量开发微卫星标记。  相似文献   

3.
桉树EST序列中微卫星含量及相关特征   总被引:6,自引:0,他引:6  
通过对桉树属(Eucalyptus)的10 000条EST序列进行分析, 在其中的1 499条序列上共发现1 775个微卫星重复序列。含有微卫星的EST序列约占序列总数的15%。此外, 还发现桉树EST序列所含微卫星长度的变异速率与重复单元长度呈负相关; 微卫星的丰度与重复单元长度也呈负相关(三碱基重复微卫星除外)。在桉树EST序列中, 重复单元长度为三碱基的微卫星最为丰富。三碱基重复单元微卫星的过度富集可能是由于遗传密码选择所致。在微卫星的丰度及长度变异方面, 桉树EST序列与杨树(Populus trichocarpa)基因组注释的转录序列随重复单元长度的变化呈现出相同的规律, 但桉树EST序列中微卫星频率及三碱基重复微卫星的含量显著偏低, 推测含微卫星的基因表达丰度极有可能低于不含微卫星的基因。通过对发现的所有微卫星位点进行引物设计, 并对设计的引物进行PCR检测, 结果表明所设计的引物具有极高的扩增成功率。  相似文献   

4.
通过对桉树属(Eucalyptus)的10000条EST序列进行分析,在其中的1499条序列上共发现1775个微卫星重复序列。含有微卫星的EST序列约占序列总数的15%。此外,还发现桉树EST序列所含微卫星长度的变异速率与重复单元长度呈负相关;微卫星的丰度与重复单元长度也呈负相关(三碱基重复微卫星除外)。在桉树EST序列中,重复单元长度为三碱基的微卫星最为丰富。三碱基重复单元微卫星的过度富集可能是由于遗传密码选择所致。在微卫星的丰度及长度变异方面,桉树EST序列与杨树(Populus trichocarpa)基因组注释的转录序列随重复单元长度的变化呈现出相同的规律,但桉树EST序列中微卫星频率及三碱基重复微卫星的含量显著偏低,推测含微卫星的基因表达丰度极有可能低于不含微卫星的基因。通过对发现的所有微卫星位点进行引物设计,并对设计的引物进行PCR检测,结果表明所设计的引物具有极高的扩增成功率。  相似文献   

5.
叶城沙蜥Phrynocephalus axillaris是我国特有的一种小型爬行动物,广泛分布于新疆塔里木盆地、吐鲁番-哈密盆地和甘肃敦煌盆地。本研究利用Roche 454 GS FLX高通量测序技术进行叶城沙蜥微卫星位点筛选,获得了91 190条高质量序列。用Krait搜索微卫星位点,共得到1~6个碱基重复类型的完美型微卫星序列29 890个。不同类型微卫星中,单碱基重复类型数目最多,有14 630个,占总数的48. 95%,其次是二碱基,约占28. 60%,四碱基、三碱基、五碱基和六碱基分别占10. 73%、10. 48%、0. 92%和0. 32%。二碱基微卫星中AC重复类型数量最多,三碱基、四碱基、五碱基和六碱基中分别是ATC、AAAT、AAAAT和AATCCC。叶城沙蜥完美型微卫星中数量最多的11种重复拷贝类型分别为C、A、AC、AG、AAAT、ATC、AT、AAT、ATAG、AGG和AAC。本研究深化了对叶城沙蜥基因组的了解,并为以后开发和筛选大量高质量微卫星标记提供了数据支持,也为利用微卫星标记研究叶城沙蜥种群遗传结构和谱系地理模式奠定了基础。  相似文献   

6.
本研究利用已公布的二斑叶螨Tetranychus urticae和肩突硬蜱Ixodes scapularis的全基因组测序结果,对其基因组中的微卫星序列进行了系统分析和比较。结果表明:在二斑叶螨基因组中共找到微卫星7934个,出现频率为1/11.45kb,占全基因组碱基总数的0.16%,其中三碱基重复微卫星最多,占总数的72.83%;在肩突硬蜱基因组中共找到550629个微卫星,出现频率为1/3.21kb,占全基因组碱基总数的0.57%,其中单碱基重复微卫星最多,占总数的73.74%。另外,肩突硬蜱基因组中微卫星的重复次数普遍高于二斑叶螨基因组中微卫星的重复次数,二斑叶螨基因组中微卫星的GC含量(34.10%)明显高于肩突硬蜱(24.35%)。微卫星家族方面,二斑叶螨基因组倾向拥有更多的唯一序列(P<0.0001)。A、T、AG、TC、TG、GAT、ATTT、AATA是两个物种共有的常见核心重复序列。  相似文献   

7.
棘腹蛙Paa boulengeri的遗传研究和基因组信息比较匮乏,致使可有效利用的分子标记非常有限。以棘腹蛙RNA-seq高通量测序数据为基础进行微卫星分子标记的大规模发掘和特征分析,结果显示:在121.6 Mb的棘腹蛙转录组序列中发现微卫星位点3165个,包含于3034条Contig序列中。在筛选到的1~6碱基重复核心的微卫星中,单碱基重复核心的比例最高,之后为三碱基、二碱基、四碱基、六碱基和五碱基重复核心,分别占29.0%、25.2%、21.7%、10.0%、10.0%和3.0%。其中A/T、AC/GT、AGG/CCT、ACAT/ATCT、AAAAT/ATTTT和AAAAAG/CTTTTT分别是单碱基、二碱基、三碱基、四碱基、五碱基、六碱基重复类型中对应的优势重复单元。棘腹蛙编码区微卫星多为重复长度小于24 bp的短序列,长度大于24 bp的微卫星仅占总数的0.92%。对编码区微卫星的侧翼序列分析发现,微卫星侧翼序列的GC含量显著低于转录组整体GC含量,且在含有微卫星上下游侧翼序列的Contig中,71.9%的序列可以设计特异引物扩增出含有微卫星序列的位点。研究结果为棘腹蛙的遗传研究和分子系统地理学研究提供了丰富的序列信息和标记资源。  相似文献   

8.
为了有效地保护四川山鹧鸪Arborophila rufipectus这一中国特有珍稀濒危鸟类,本研究采用454 GS FLX对该物种基因组测序,首次利用微卫星搜索软件搜索并初步统计和分析基因组微卫星序列,共搜索到l~6个碱基重复类型的完美型微卫星335 263个。不同类型微卫星中,单碱基重复类型数目最多,为197 913个,约占总数的59.03%,其次是四碱基、三碱基、六碱基、二碱基和五碱基,分别约占微卫星总数的13.59%、8.39%、7.55%、6.49%和4.95%。单碱基微卫星中A重复类型数量最多,两碱基中AC最多,三碱基中AAC,四碱基中AAAC最多,五碱基中AAACA最多,六碱基中AGGGTT最多。A、AGGGTT、AAAC、AC、AAAT、AAC、C、AG、AAAG、AAACA、AAT、AGG、AT、AGC、AAGG、CCG是在所搜索到的四川山鹧鸪微卫星中数量最多的16种重复拷贝类型。本研究深化了对四川山鹧鸪基因组的认识和了解,并为以后开发和筛选大量高质量微卫星标记提供数据支持,也为利用微卫星标记研究更加有效地保护和管理四川山鹧鸪这一珍稀濒危动物奠定了基础。  相似文献   

9.
用磁珠富集法构建了岩原鲤Procypris rabaudi AC重复和GATA重复的微卫星富集文库.采用PCR方法分别以人工合成的oligoA和探针(AC)12或(GATA)6为引物筛选含有微卫星的阳性克隆.(AC)n 富集库和(GATA)n富集库的阳性克隆率分别为30%和7%左右.对40个AC重复的阳性克隆和30个GATA重复的阳性克隆测序,共获得61个微卫星序列,其中包含了一个三碱基重复(TGA)的微卫星序列.选择设计了19对AC重复和16对GATA重复的微卫星引物以及1对TGA重复的微卫星引物,通过PCR优化,共有20对引物能够产生稳定、清晰的目的产物带.为了检测获得的岩原鲤微卫星座位是否能用于近缘物种的研究,我们将20对岩原鲤微卫星引物用于中华倒刺鲃Spinibarbus sinensis基因组DNA PCR扩增,有60%的引物对能产生特异性的目的条带.本研究获得的20个岩原鲤微卫星座位可以用于岩原鲤及近缘物种的遗传多样性、种群遗传结构等的进一步研究.  相似文献   

10.
为了获得适于三叶木通遗传多样性和遗传结构研究的微卫星分子标记,该研究采用磁珠富集法构建了三叶木通微卫星富集文库。结果表明:在150个阳性克隆中发现了70个微卫星位点,富集效率为46.67%,其中含双碱基重复单元的序列占比为79.37%,三碱基和四碱基重复含有量较少。共设计引物63对,其中筛选出16对高多态引物,对1个三叶木通自然居群48个个体进行了遗传分析,结果显示位点的等位基因数为10~22个,观察杂合度和期望杂合度分别为0.370~0.792和0.724~0.936,多态性信息指数为0.725~0.919,表明以上引物均为高多态性引物。其中,12个位点偏离哈迪-温伯格平衡,呈现出纯合子过剩状态,这可能与哑等位基因和其它因素有关。综上结果表明,该研究所开发的16对引物能够用于三叶木通遗传多样性和遗传结构评价工作。  相似文献   

11.
基于转录组数据的桔小实蝇微卫星位点信息分析   总被引:3,自引:0,他引:3  
以桔小实蝇为材料,从其转录组数据库中筛选功能微卫星(EST-SSR)序列,并进行SSR位点的信息分析.共获得1890个EST-SSR位点,可用于引物设计的SSR数为1296个.EST-SSR平均分布频率为1/10.21 kb,但这种分布频率在不同重复类型SSR之间相差很大.其中,三碱基重复SSR在该种昆虫的EST-SSR中出现的频率最高,结合其他文献推断三碱基重复可能是所有昆虫EST-SSR的优势类型.本文共设计了42对桔小实蝇EST-SSR引物,其中有18对引物可以扩增得到预期大小的条带.最后,探讨了基于转录组数据发掘昆虫SSR的前景和挑战,以及进行转录组EST-SSR筛选时应注意的问题.
  相似文献   

12.
亚麻EST-SSR信息分析与标记开发   总被引:3,自引:0,他引:3  
与基因组SSR相比,以EST为基础的EST-SSR分子标记具有自身的优点。本研究从11240条亚麻(Linum sitatissmum L.)EST序列中检索出877条含有SSR的序列,其出现频率为7.8%。其中以三核苷酸重复出现的频率最高,占总SSR序列的60.1%;其次是二核苷酸重复,占21.9%;四、五和六核苷酸重复占18%。根据这些含SSR的EST序列共设计了73对SSR引物,在8份亚麻材料间通过PCR扩增检测,有63对引物扩增出清晰条带,引物可用率86.3%;有17对引物在8份亚麻材料间显现出多态性,占可扩增引物的26.3%。  相似文献   

13.
基于转录组数据高通量发掘扶桑绵粉蚧微卫星引物   总被引:7,自引:0,他引:7  
罗梅  张鹤  宾淑英  林进添 《昆虫学报》2014,57(4):395-400
【目的】扶桑绵粉蚧Phenacoccus solenopsis Tinsley是我国重要的检疫性害虫。简单重复序列(simple sequence repeat,SSR)研究在遗传图谱和物理图谱的构建、分子标记辅助育种、品种鉴定、基因定位、遗传多样性、动植物分类和进化等方面具有重要意义。筛选的SSR引物将为扶桑绵粉蚧遗传多样性分析、进化分析及入侵生物学等奠定基础。【方法】利用高通量搜索的方法对扶桑绵粉蚧转录组中28 120条unigenes的数据进行搜索。【结果】共找到1 781个SSR位点。扶桑绵粉蚧转录组中SSRs的主要重复类型是单核苷酸重复,占SSR总数的89.44%;其次是三核苷酸重复,占SSR总数的7.52%。单核苷酸重复里主要是A/T基序,占了总量的87.42%。基于筛选的SSRs,运用Primer 3软件进行引物的批量设计,共有481个unigenes成功设计引物,共设计出1 228对引物。【结论】研究表明利用扶桑绵粉蚧转录组数据开发SSR标记是可行的,本研究开发的引物将为扶桑绵粉蚧遗传多样性分析、进化分析及入侵生物学等奠定基础。  相似文献   

14.
该研究主要开发筛选适用于杂交兰的EST-SSR引物,为杂交兰种质资源评价和遗传变异研究等提供可靠的分子标记。该研究对杂交兰进行转录组高通量测序,挖掘SSR位点和开发EST-SSR标记,并对不同种质的遗传多样性进行分析。结果表明,从31724条杂交兰Unigene中检测出18603个SSR位点,SSR出现频率为58.64%;SSR位点中的主导类型是单核苷酸重复,占总SSR的65.10%,其次是二核苷酸(23.56%)和三核苷酸(10.76%)重复;优势重复基元为A/T、AG/CT、AT/AT和AAG/CTT,分别占总位点的64.72%、13.74%、8.19%和2.51%。利用Primer Premier 5.0共设计了565对SSR引物,从筛选出的64对有效扩增引物中随机选择28对引物,对40份杂交兰种质进行多态性验证与遗传关系分析,其中16对(占57.14%)引物表现出可重复的高多态性,平均多态信息量(PIC)达0.789。基于扩增的多态性SSR信息,40份种质资源可聚为4类,聚类结果与其遗传背景基本一致。该研究印证了转录组测序获得的Unigene是SSR标记开发的有效来源,开发的EST-SSR引物可为杂交兰及近缘种的良种鉴别、遗传图谱构建、分子标记辅助育种及功能基因挖掘等提供有价值的候选标记。  相似文献   

15.
【背景】韭菜迟眼蕈蚊是我国重要的农业害虫,然而它的遗传资源有限。本研究旨在开发韭菜迟眼蕈蚊EST-SSR标记,为研究不同地区的韭菜迟眼蕈蚊种群结构和遗传多样性奠定基础。【方法】从韭菜迟眼蕈蚊的表达序列标签(EST序列)中设计16对简单重复序列(SSR)引物,进一步筛选出9对具有多态性的SSR引物。【结果】从42095条unigene中确定了3383个SSR位点。利用查找到的SSR位点共设计出16对引物,进一步检测筛选发现9对引物具有多态性,引物的每个位点平均有3.33个等位基因。利用9对引物对30头韭菜迟眼蕈蚊进行检测,共获得30个等位基因,观测杂合度和期望杂合度的范围分别为0.0000~0.6875和0.0370~0.6877;其中,9个位点中有5个位点显著偏离Hardy-Weinberg平衡。【结论与意义】本研究成功从迟眼蕈蚊EST序列中筛选出9个具有多态性的微卫星位点,这为进一步分析该害虫种群的遗传结构和遗传多样性奠定了基础。  相似文献   

16.
The tea plant (Camellia sinensis (L.) O. Kuntze) is one of the most popular non-alcoholic beverage crops worldwide. The availability of complete genome sequences for the Camellia sinensis var. ‘Shuchazao’ has provided the opportunity to identify all types of simple sequence repeat (SSR) markers by genome-wide scan. In this study, a total of 667,980 SSRs were identified in the ~?3.08 Gb genome, with an overall density of 216.88 SSRs/Mb. Dinucleotide repeats were predominant among microsatellites (72.25%), followed by trinucleotide repeats (15.35%), while the remaining SSRs accounted for less than 13%. The motif AG/CT (49.96%) and AT/TA (40.14%) were the most and the second most abundant among all identified SSR motifs, respectively; meanwhile, AAT/ATT (41.29%) and AAAT/ATTT (67.47%) were the most common among trinucleotides and tetranucleotides, respectively. A total of 300 primer pairs were designed to screen six tea cultivars for polymorphisms of SSR markers using the five selected repeat types of microsatellite sequences. The resulting 96 SSR markers that yielded polymorphic and unambiguous bands were further deployed on 47 tea cultivars for genetic diversity assessment, demonstrating high polymorphism of these SSR markers. Remarkably, the dendrogram revealed that the phylogenetic relationships among these tea cultivars are highly consistent with their genetic backgrounds or places of origin. The identified genome-wide SSRs and newly developed SSR markers will provide a powerful means for genetic researches in tea plant, including genetic diversity and evolutionary origin analysis, fingerprinting, QTL mapping, and marker-assisted selection for breeding.  相似文献   

17.
Chinese jujube (Ziziphus jujuba), an economically important species in the Rhamnaceae family, is a popular fruit tree in Asia. Here, we surveyed and characterized simple sequence repeats (SSRs) in the jujube genome. A total of 436,676 SSR loci were identified, with an average distance of 0.93 Kb between the loci. A large proportion of the SSRs included mononucleotide, dinucleotide and trinucleotide repeat motifs, which accounted for 64.87%, 24.40%, and 8.74% of all repeats, respectively. Among the mononucleotide repeats, A/T was the most common, whereas AT/TA was the most common dinucleotide repeat. A total of 30,565 primer pairs were successfully designed and screened using a series of criteria. Moreover, 725 of 1,000 randomly selected primer pairs were effective among 6 cultivars, and 511 of these primer pairs were polymorphic. Sequencing the amplicons of two SSRs across three jujube cultivars revealed variations in the repeats. The transferability of jujube SSR primers proved that 35/64 SSRs could be transferred across family boundary. Using jujube SSR primers, clustering analysis results from 15 species were highly consistent with the Angiosperm Phylogeny Group (APGIII) System. The genome-wide characterization of SSRs in Chinese jujube is very valuable for whole-genome characterization and marker-assisted selection in jujube breeding. In addition, the transferability of jujube SSR primers could provide a solid foundation for their further utilization.  相似文献   

18.
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Faba bean (Vicia faba L.) is an important food legume crop with a huge genome. Development of genetic markers for faba bean is important to study diversity and for molecular breeding. In this study, we used Next Generation Sequencing (NGS) technology for the development of genomic simple sequence repeat (SSR) markers. A total of 14,027,500 sequence reads were obtained comprising 4,208 Mb. From these reads, 56,063 contigs were assembled (16,367 Mb) and 2138 SSRs were identified. Mono and dinucleotides were the most abundant, accounting for 57.5 % and 20.9 % of all SSR repeats, respectively. A total of 430 primer pairs were designed from contigs larger than 350 nucleotides and 50 primers pairs were tested for validation of SSR locus amplification. Nearly all (96 %) of the markers were found to produce clear amplicons and to be reproducible. Thirty-nine SSR markers were then applied to 46 faba bean accessions from worldwide origins, resulting in 161 alleles with 87.5 % polymorphism, and an average of 4.1 alleles per marker. Gene diversity (GD) of the markers ranged from 0 to 0.48 with an average of 0.27. Testing of the markers showed that they were useful in determining genetic relationships and population structure in faba bean accessions.  相似文献   

20.
Opium poppy (Papaver somniferum L.) is an important pharmaceutical crop with very few genetic marker resources. To expand these resources, we sequenced genomic DNA using pyrosequencing technology and examined the DNA sequences for simple sequence repeats (SSRs). A total of 1,244,412 sequence reads were obtained covering 474 Mb. Approximately half of the reads (52 %) were assembled into 166,724 contigs representing 105 Mb of the opium poppy genome. A total of 23,283 non-redundant SSRs were identified in 18,944 contigs (11.3 % of total contigs). Trinucleotide and tetranucleotide repeats were the most abundant SSR repeats, accounting for 49.0 and 27.9 % of all SSRs, respectively. The AAG/TTC repeat was the most abundant trinucleotide repeat, representing 19.7 % of trinucleotide repeats. Other SSR repeat types were AT-rich. A total of 23,126 primer pairs (98.7 % of total SSRs) were designed to amplify SSRs. Fifty-three genomic SSR markers were tested in 37 opium poppy accessions and seven Papaver species for determination of polymorphism and transferability. Intraspecific polymorphism information content (PIC) values of the genomic SSR markers were intermediate, with an average 0.17, while the interspecific average PIC value was slightly higher, 0.19. All markers showed at least 88 % transferability among related species. This study increases sequence coverage of the opium poppy genome by sevenfold and the number of opium poppy-specific SSR markers by sixfold. This is the first report of the development of genomic SSR markers in opium poppy, and the genomic SSR markers developed in this study will be useful in diversity, identification, mapping and breeding studies in opium poppy.  相似文献   

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