猪H-FABP基因PCR-SSCP分析

应用PCR-SSCP方法分析了H-FABP基因在山西白猪、马身猪、大白猪、长白猪和杜洛克猪5个猪种的多态性。结果表明:在H-FABP基因内含子1中发现了多态位点,该位点上具有两个等位基因A和B,马身猪BB基因型频率最高,B等位基因频率明显高于A等位基因频率;其余4个猪种AA基因型频率最高。序列测定的结果表明,SSCP的变异是由碱基C→T的替换造成的。     

PCR－SSCP检测肺癌细胞p53基因点突变

应用溴化乙锭(EB)染色的PCR-SSCP技术对10例非小细胞性肺癌组织标本p53基因外显子5～8进行分析,其中1例在外显子5～6;1例在外显子7;2例在外显子8发现异常电泳带.对1例经SSCP检测异常的p53基因进行核酸序列分析,发现第280位密码子由AGA变成ACA,其编码的氨基酸由丝氨酸变成半胱氨酸.结果证实:非小细胞性肺癌与p53基因突变有关;EB法PCR-SSCP技术是一种简便、可靠的点突变检测法.     

四个牦牛品种MC1R基因部分序列的多态性研究

为探索4个牦牛品种MC1R基因多态性的相关信息,选取甘南牦牛、天祝白牦牛、青海高原牦牛、大通牦牛4个品种共408头个体为研究对象,采用PCR-SSCP方法分析牦牛MC1R基因部分序列的基因多态性。结果表明,与GenBank中牛MCIR基因序列(登录号:AF445641.1)比对发现,该扩增片段在3 891 bp处发生C→G的突变,在3 912 bp处发生T→C的突变,共发现CC、DD、EE、CD、CE和DE 6种基因型。4个牦牛品种中CD、CE和DE 3种基因型在青海高原牦牛和大通牦牛中占主要优势,这3种基因型频率总和在青海高原牦牛和大通牦牛群体中分别是0.778和0.781。DD和CD两基因型是甘南牦牛群里中的优势基因型,其基因型频率分别是0.351和0.328。天祝白牦牛中优势基因型是DD,其基因型频率是0.500。D等位基因是4个地方品种牦牛中的优势等位基因。4个地方品种在该基因座上都处于Hardy-Weinberg平衡状态(P>0.05)。青海高原牦牛和大通牦牛两个群体处于高度多态(PIC>0.5),甘南牦牛和天祝白牦牛处于中度多态(0.25相似文献   

藏獒MC1R基因多态性与毛色表型的关联研究

目的:通过检测藏獒黑素皮质激素受体1(MC1R)基因的单链构象多态性(SSCP)在不同毛色群体中的分布,探讨MC1R基因多态性与毛色表型的相关性。方法:采用DNA测序技术,选择不同毛色藏獒的DNA为样本,根据GenBank发布的荷斯坦牛MC1R基因序列设计一对引物,采用PCR-SSCP技术分析MC1R基因在藏獒中的SSCP。结果:MC1R基因在藏獒中具有PCR-SSCP多态性,分别检测到3种基因型(AA、AB和BB);对MC1R基因多态性片段DNA克隆测序后发现,MC1R基因在编码区第313位存在单碱基突变(G→A),该突变导致第105位氨基酸发生由丙氨酸向苏氨酸的改变(T105A)。结论:MC1R基因的多态性与毛色性状不存在显著的相关性。     

PCR-SSCP技术在假丝酵母属菌种鉴别中的应用

选取中国工业微生物菌种保藏管理中心(CICC)保藏的假丝酵母属的7个种30株菌, 对其rDNA的ITS1区及ITS2区进行了PCR-SSCP指纹图谱分析, 结果表明在假丝酵母属种水平的区分鉴定中, ITS1区与ITS2区的PCR-SSCP图谱均能对本研究所选7个种的菌株进行显著区分, 比较两个区段的PCR-SSCP图谱及鉴别效果, 发现ITS2区的应用效果要优于ITS1区。     

Two genetically distinct units of Sinomanglietia glauca （Magnoliaceae） detected by chloroplast PCR-SSCP

Sinomanglietia glauca is a critically endangered species described from Jiangxi Province in the 1990s. Recently two populations were discovered from Yongshun County of west Hunan Province, about 450 km away from those in Jiangxi. Because of the new findings and the poor reproducibility inherent to RAPD and ISSR markers of previous studies, the population structure of this rare species was reanalyzed with chloroplast PCR-SSCP （single-stranded conformation polymorphism）, including all of four recorded populations. The results showed that two distinct haplotypes characterized Jiangxi and Hunan populations separately, with no genetic variation occurring within regions. We postulated that this surprising pattern might result from habitat fragmenta- tion and demographic bottlenecks during and/or after the Quaternary glaciation. On the basis of the pronounced genetic structure, two evolutionarily significant units （ESUs） were recommended for effective conservation of S. glauca.     

浓香型白酒窖池细菌群落

利用PCR-SSCP技术研究了不同窖龄浓香型白酒窖池细菌群落的变化规律,结果发现:(1)所有窖泥样品均出现9-22条较清晰的条带,其中均表现出较高优势度的条带7条,但各样品优势条带的变化规律不同;(2)所有窖泥样品平均生物多样性指数都在1.93-2.82之间,随着窖龄的增加,相同位置样品的多样性指数总体上呈递增趋势;(3)同一窖池不同位置样品的PCR-SSCP图谱相似性指数较高,在0.63-1.00之间,不同窖龄窖池的SSCP图谱相似性指数较低,在0.34-0.76之间。     

甘肃现代肉羊新品种群羊GH基因外显子1多态性与体重关联分析

根据GenBank发表的绵羊生长激素(GH)基因外显子1的序列设计一对引物,采用PCR-SSCP技术分析GH基因外显子1在甘肃现代肉羊新品种选育群羊中的单核苷酸多态性,并与3月龄前的体重进行关联分析。结果表明,GH基因外显子1在新品种群羊中存在多态性,检测到两种基因型(AA、AB),其301bp处有一个T/A突变和305bp处有一个G/A突变,初生重、1月、2月、3月龄体重AA、AB型都无显著性差异(P>0.05),但3月龄AB型个体的体重相对于AA型偏高,由此初步推断GH基因可能是影响绵羊体重性状的主基因或与主基因相连锁,可用以对绵羊体重性状进行标记辅助选择。     

五指山猪GH、IGFBP3基因SNPs检测及与生长性状的关联分析

以五指山猪为试验材料,采用PCR-SSCP和测序相结合技术,对GH基因和IGFBP3基因进行多态性检测,并分析其与生长性状(体质量,体高,体长和胸围)的相关性。结果表明,GH基因第2外显子存在一处G→A转换,属沉默突变,该位点与生长性状关联分析显示,BB基因型的体重显著高于AA基因型和AB基因型;IGFBP3基因第2外显子存在一处G→C颠换,属沉默突变,该位点与生长性状关联分析显示,AA基因型的体高显著高于BB基因型;IGFBP3基因第4内含子存在一处碱基C缺失,该位点与生长性状关联分析显示,AA基因型体重显著高于AB基因型和BB基因型。研究将为五指山猪生长发育规律、系统选育及矮小机制等方面研究提供了遗传学依据。     

Bacterial diversity in maize rhizospheres: conclusions on the use of genetic profiles based on PCR-amplified partial small subunit rRNA genes in ecological studies

A cultivation-independent approach based on polymerase chain reaction (PCR)-amplified partial small subunit rRNA genes and genetic profiling by single-strand conformation polymorphism (SSCP) was used to characterize the bacterial diversity inhabiting the rhizosphere of maize plants grown on an agricultural field. The community structures of two cultivars, a genetically engineered and a nonengineered variety, different herbicide regimes and soil tillage were compared with each other at two sampling dates. SSCP-profiles were generated with DNA from bacterial cell consortia with primers hybridizing to evolutionarily highly conserved rRNA gene regions. On silver-stained gels, each profile consisted of approx. 50 distinguishable bands. Similarity analyses of patterns recorded by digital image analyses could not detect any difference between cultivars or treatments that was greater than the variability between replicates. A total of 54 sequences recovered from different bands were identified and grouped into operational taxonomical units (OTUs). Surprisingly, only five of 40 OTUs contained sequences of both samplings. Three different bands from a profile were selected to test whether this small overlap was due to an incomplete recovery of sequences. From a faint band, two different OTUs were found when 12 clones were analysed, and from two strong bands 24 and 22 OTUs were detected from a total of 26 and 36 clones, respectively. The OTUs belonged to phylogenetically different groups of bacteria. Gene probes that were developed to target different bands of the profiles, however, indicated in Southern blot analyses that patterns between treatments, replicates and samplings, and even from two different growing seasons were highly conserved. Our study demonstrates that community profiles can consist of more sequences than detectable by staining and that gene probes in Southern blot can be a useful control to investigate the composition of microbial communities by genetic profiles.