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1.
近交系小鼠微卫星DNA多态性的研究   总被引:22,自引:2,他引:20  
随机选择位于小鼠不同染色体上的微卫星引物42对,用PCR技术对C3H、C57、BALB/c、DBA、TA2、T739、B615、BACB/c-nu-nu和SCID等9种实验室常用近交系小鼠微卫星DNA多态性进行了研究.结果显示有信息的40对引物中,9种近交系小鼠在各基因座上均出现一条清晰条带,28个基因座表现为多态性.其中D3Mit22、D7Nds1、D11Mit12、D12Nds2、D15Mit17、D16Mit3、D16Mit4基因座表现为显著多态性.T739、B615和TA2的遗传背景相近,其相似系数分别为90%和85%;其次为TA2、SCID和B615,其相似系数分别为80%和82.5%.结果表明所检测的小鼠符合近交要求,筛选出的引物能典型地反映9个近交系小鼠的品系特异性和遗传背景,可用于常规检测小鼠品系来源和遗传背景等.  相似文献   

2.
近交系小鼠微卫星DNA多态性的研究   总被引:8,自引:0,他引:8  
随机选择位于小鼠不同染色体上的微卫星引物42对,用PCR技术对C3H、C57、BALB/c、DBA、TA2、T739、B615、BACB/c-nu-nu和SCID等9种实验室常用近交系小鼠微卫星DNA多态性进行了研究。结果显示有信息的40对引物中,9种近交系小鼠在各基因座上均出现一条清晰条带,28个基因座表现为多态性。其中D3Mit22、D7Nds1、D11Mit12、D12Nds2、D15Mit17、D16Mit3、D16Mit4基因座表现为显著多态性。T739、B615和TA2的遗传背景相近,其相似系数分别为90%和85%;其次为TA2、SCID和B615,其相似系数分别为80%和82.5%。结果表明所检测的小鼠符合近交要求,筛选出的引物能典型地反映9个近交系小鼠的品系特异性和遗传背景,可用于常规检测小鼠品系来源和遗传背景等。 Abstract:Forty-two microsatellites DNA loci on different chromosomes in nine kinds of inbred strain mice including C3H,C57,BALB/c,DBA,TA2,T739,B615,BALB/c-nu-nu and SCID were investigated by PCR analysis.It showed that all these mice tested display single allelic gene band with forty pairs of informative primers.Twenty-eight loci are polymorphisms,among which the polymorphisms of D3Mit22,D7Nds1,D11Mit12,D12Nds2,D15Mit17,D16Mit3,and D16Mit4 loci are significant.The genetic background of T739 was similarity with that of B615 and TA2 ,the similarity indices were 90% and 85% respectively;and that of TA2 was similarity with SCID and B615,the similarity indices were 80% and 82.5%.These results suggest that these mice tested meet the request of inbred strain.Screened primers showing marked polymorphisms topically reflect the speciality of strains and genetic backgrounds,which could be used in determining the strains origin and genetic background of mice.  相似文献   

3.
目的利用多态性微卫星DNA位点分析PLCε基因敲除小鼠的遗传特性。方法用所筛选的15个微卫星DNA位点对28只PLCε基因敲除小鼠的DNA进行了PCR扩增,通过基因片段大小来分析群体的遗传多样性。结果 13个微卫星DNA位点中(D1Mit365、D3Mit51、D4Mit235、D6Mit102、D7Mit281、D8Mit113、D9Mit23、D10Mit180、D13Mit88、D16Mit145、D17Mit36、D18Mit94、D19Mit97)每个位点的28只小鼠DNA片段泳动距离一致,呈现单态性,表明该群体符合近交系的遗传特性;而利用Dq(敲基因型)和Dy(野生型)两个位点对28只小鼠的PCR扩增结果进行了鉴别分析,其中敲除基因型小鼠为6只;野生型为7只;杂合型为15只。结论利用微卫星标记技术可以对群体进行遗传质量监测,并能有效地鉴别不同的基因型,为小鼠的遗传质量监测提供了一种可行的方法。  相似文献   

4.
小鼠39个微卫星的PCR条件及其运用   总被引:14,自引:3,他引:11  
目的探索小鼠基因组39个微卫星的PCR条件,评价微卫星在小鼠遗传检测中的运用.方法采用梯度法探索39个微卫星的PCR条件;选择本中心不同来源及引种时间的C57BL/6、BALB/c、DBA/2J、CBA/N、FVB/NJ、ICR共6个品系(8个组)小鼠,每组采用10只个体的鼠尾,提取DNA并混合成DNA池,用39个微卫星扩增后电泳观察、比较种系纯度.结果小鼠微卫星的PCR条件差异较大,Mg2+浓度多数在1.5 mmol/L左右,退火温度多数在59℃左右.在6个品系小鼠的39个微卫星位点中,C57BL/6、BALB/c、DBA/2J都是纯合的; 其余品系有1~3个杂合位点. BALB/c在D5Mitl68、D8Mit320、D13Mit262三个位点,DBA/2J在D14Mit205位点与数据库记录有差异.结论本研究为小鼠39个微卫星提供了候选的PCR条件,并对6个品系小鼠的微卫星概貌及微卫星的运用价值进行了探讨.  相似文献   

5.
应用RAPD方法对近交系小鼠进行遗传检测的研究   总被引:11,自引:1,他引:10  
目的 为实验室日常检测近交系小鼠的遗传背景提供一种分子生物学方法。方法 用 6条随机引物对 6个品系近交系小鼠基因组DNA进行PCR扩增。结果  6条随机引物中p2、p3、p5和p6四引物扩增的条带差异较为明显。结论 RAPD方法是一种有效的近交系小鼠遗传检测手段  相似文献   

6.
应用微卫星分子标记对昆明小鼠(KM)封闭群相隔10代的两个群体(分别命名为A9和A19)进行遗传背景分析,共设计位于小鼠7条染色体上的7对微卫星引物用于实验研究,选取具有多态性的一个微卫星位点D3Mit22进行详细分析.结果表明:所研究的位点D3Mit22在两个群体共发现2个不同的等位基因,3种不同的基因型,其中A9代有3种不同的基因型,即AB,AA,BB.A19代有两种不同的基因型,即AB,BB.进一步埘不同的微卫星位点克隆测序,分析了该位点的DNA分子特性.对封闭群小鼠检测方法的建立及保持封闭群小鼠的遗传稳定性提供了重要的分子数据.  相似文献   

7.
ENU诱导获得一种短尾小鼠及其突变基因的初步定位   总被引:2,自引:1,他引:1  
用一种化学诱变剂ENU(乙酰基亚硝基脲 )腹腔注射 3 0只 8~ 1 0周龄C5 7BL 6J(简称B6)雄鼠 (G0代 ) ,6周后与同品系正常母鼠配种繁殖后代 (G1代 )小鼠 3 5 1只。对其后代进行筛选获得一种可遗传的显性短尾突变小鼠。为了定位该突变基因 ,运用平均分布于B6和DBA 2 (简称D2 )小鼠常染色体而在这两者间又有差异的 3 9个微卫星对突变小鼠的 (D2×B6)F1代短尾突变小鼠回交D2得到的有短尾表型的[(B6×D2 )F1×D2 ]F2 代小鼠进行基因组扫描。反向运用经典的位置候选基因法 ,将短尾突变基因定位于 1 7号染色体 ,与D1 7Mit3 3的LOD值为 9 0 8。选用该染色体上与短尾表型相关基因Brachyury (T)最近的微卫星D1 7Mit1 43引物扩增 ,在 1 0 9只F2 代短尾小鼠中未发生一例交换 ,表明Brachyury基因是本例短尾突变强有力的候选基因。  相似文献   

8.
两种白斑小鼠突变基因的染色体定位   总被引:5,自引:1,他引:4  
以本中心ENU诱变获得的两种白斑突变小鼠W-4Bao与Kitl-1Bao为研究对象[均为C57BL/6J(B6)背景],遗传试验表明它们都为单基因显性遗传,W-4Bao及Kitl-1Bao突变基因纯合子小鼠的表型分别为全白色及“黑头白”;将白斑杂合子小鼠与DBA/2(D2)交配获得具有白斑表型的F1小鼠,F1小鼠再回交D2繁殖[(B6×D2)F1×D2]F2小鼠,利用微卫星标记对F2代小鼠进行连锁分析。结果发现W-4Bao与微卫星D5Mit356、D5Mit308之间的LOD值分别为56.82、51.50,从而把该突变基因定位于第5号染色体D5Mit356与D5Mit308之间;Kitl-1Bao与微卫星D10Mit70、D10Mit68之间的LOD值分别为27.37、21.20,从而把该突变基因定位于第10号染色体上D10Mit70与D10Mit68之间。经过检索小鼠基因组数据库确认它们的候选基因分别为kit及kitl。  相似文献   

9.
四川农业大学小麦研究所侯永翠、郑有良、魏育明等研究人员对黑麦遗传多样性课题作了研究。他们采用随机扩增多态性DNA(RAPD)标记 ,对黑麦属 (SecaleL) 7个品种共 1 2份材料进行了遗传多样性检测 ,发现被检测材料间RAPD标记多态性较高 ,在 4 0个随机引物中 ,有 2 5个引物约占整个的 6 2 .5 %的扩增产物具有多态性。这 2 5个中共扩增出 1 6 7条带 ,其中 89条带约占 5 3.2 %具有多态性 ,每个引物可扩增出 1~ 1 0条多态性带 ,平均为 3~ 6条。RAPD标记遗传距离GD变异范围为 0 .1 382~ 0 .4 5 1 2 ,平均为 0 .2 71 2。通过聚类分析表…  相似文献   

10.
金银花五个品系的RAPD分析及DNA指纹图谱的建立   总被引:5,自引:0,他引:5  
运用RAPD技术,对5个金银花品系进行遗传多样性研究并构建这5个金银花品系的DNA指纹图谱。从80个引物中筛选出25个带纹清晰,多态性好的引物用于实验。其中,引物SBSD06的扩增条带可以清楚明确区分5个品系,建立其DNA指纹图谱。在清晰、稳定出现的170条带中,153条带具有多态性。按UPGMA法进行聚类分析,计算其遗传相似系数,结果显示,金银花5个品系聚为两类,与其形态学分类结果相符。  相似文献   

11.
10个品系小鼠的RAPD 分析   总被引:2,自引:0,他引:2  
李淑蓉  陈意生  魏泓 《动物学报》2002,48(3):429-432
小鼠是应用最为广泛的实验动物,预先了解品系或近交系的遗传纯度或系间遗传距离,对于试验材料的选取和实验结果分析都有很大帮助.传统的实验动物遗传监测多限于基因表型的检测,检测位点在整个基因组中所占比例小,分布不均.由于RAPD方法的优势,用一系列引物可检测出覆盖整个基因组的遗传改变,在动、植物品系鉴定和遗传监测方面已取得大量成果(陈洪等,1994;沈曦等,1999),但对多品系小鼠的研究报道较少.因此,本研究选用10个常用小鼠品系,筛选较好的多态标记,建立各品系的RAPD图谱,以区分不同品系的小鼠,为今后的质量监测工作提供参照标准;同时根据RAPD扩增结果计算出各品系间的相对遗传距离,在DNA水平探讨不同品系小鼠间的亲缘关系.  相似文献   

12.
目的比较随即扩增多态性方法(RAPD)、微卫星方法(STR)与生化标记方法对近交系小鼠遗传质量检测的差异,为近交系动物遗传质量控制提供一种分子生物学方法。方法提取近交系小鼠BALB/c基因组DNA,用6条RAPD引物和20对STR引物对其进行PCR扩增,用生化标记法检测13个位点。结果在6条RAPD引物中,引物2(p2)、引物3(p3)、引物5(p5)和引物6(p6)这四条引物扩增的条带出现差异,表现为不同的RAPD图谱;在20对STR引物中,引物2、4、10和11,这四对引物扩增的条带出现差异,表现为不同的STR图谱;13个生化标记位点中,过氧化氢酶-2(Ce-2)等6个生化位点发现杂合基因。结论RAPD和STR可用于验证生化标记方法的实验结果,并用于保证近交系动物的遗传质量。  相似文献   

13.
We have established a genetic quality testing system for early stage embryos of the mouse. A method of preparation of template DNA for PCR was established using the lysis buffer (1 x PCR reaction buffer supplemented with proteinase K at a concentration of 40 microg/ml) developed by the authors. We demonstrated that two 8-cell embryos of an inbred strain provide sufficient volumes of template DNA for PCR to identify the strain of embryos using four microsatellite markers (D3Mit54, D5Mit18, D6Mit15 and D8Mit50) differentiating 13 inbred strains of mice. This system will be useful in embryo banks that have recently been established worldwide for demonstrating the genetic accuracy of a given strain prior to recovery of live animals.  相似文献   

14.
目的利用微卫星技术对辽宁省6种近交系小鼠进行遗传质量分析。方法根据Mouse Genome Database和相关文献选取10个多态信息丰富的位点和引物,进行PCR扩增和PAGE电泳,对小鼠的遗传多态性进行研究。结果不同品系小鼠同一位点的扩增结果表现出多态性,同一品系同一位点表现单态性,所有小鼠的10个位点都处于纯合状态;遗传距离分析表明,C57BL/10与C57BL/6J小鼠之间的遗传距离最近,为0.1021,遗传距离最远的是BALB/c与C57BL/10、C57BL/6J,分别为0.1635和0.1614。结论运用所筛选的10个微卫星位点可以对近交系小鼠进行遗传质量检测,说明该方法具备可行性。  相似文献   

15.
用微卫星标记技术对国内BALB/c小鼠遗传质量的分析   总被引:11,自引:1,他引:10  
陈振文  欧阳兆和  董罡  李瑞生 《遗传》2004,26(6):845-848
为了解和掌握国内BALB/c小鼠遗传质量状况,验证微卫星标记技术在近交系小鼠遗传检测中应用的可靠性,应用所筛选的小鼠不同染色体上的14个微卫星基因座,通过PCR扩增对北京、上海、沈阳、广州、长春、重庆和哈尔滨7个地区11个厂家提供的BALB/c小鼠进行遗传质量分析.结果北京、上海、哈尔滨及广州地区7家BALB/c小鼠在14个基因座均呈现一条清晰条带,且群体间呈单态性.沈阳、广州、长春和重庆4个群体有8个基因座在群体内表现杂合或呈多态性;其中沈阳和长春分别在1个基因座上表现多态性和杂合;广州另一群体有4个基因座出现杂合或多态性;重庆群体有7个基因座表现为杂合或多态性,在D10Mit180基因座与上海群体比较呈现多态性.  相似文献   

16.
PCR primers of arbitrary nucleotide sequence have identified DNA polymorphisms useful for genetic mapping in a large variety of organisms. Although technically very powerful, the use of arbitrary primers for genome mapping has the disadvantage of characterizing DNA sequences of unknown function. Thus, there is no reason to anticipate that DNA fragments amplified by use of arbitrary primers will be enriched for either transcribed or promoter sequences that may be conserved in evolution. For these reasons, we modified the arbitrarily primed PCR method by using oligonucleotide primers derived from conserved promoter elements and protein motifs. Twenty-nine of these primers were tested individually and in pairwise combinations for their ability to amplify genomic DNA from a variety of species including various inbred strains of laboratory mice and Mus spretus. Using recombinant inbred strains of mice, we determined the chromosomal location of 27 polymorphic fragments in the mouse genome. The results demonstrated that motif sequence-tagged PCR products are reliable markers for mapping the mouse genome and that motif primers can also be used for genomic fingerprinting of many divergent species.  相似文献   

17.
Zuo B  Du X  Zhao J  Yang H  Wang C  Wu Y  Lu J  Wang Y  Chen Z 《PloS one》2012,7(4):e34555
Previously, we found that the genotype of 42 out of 198 mouse microsatellite loci, which are distributed among all chromosomes except the Y chromosome, changed from monomorphism to polymorphism (CMP) in a genetically modified inbred mouse strain. In this study, we further examined whether CMP also relates to the homologous recombination in gene knockout (KO) mouse strains. The same 42 microsatellite loci were analyzed by polymerase chain reaction (PCR) in 29 KO inbred mouse strains via short tandem sequence repeat (STR) scanning and direct sequence cloning to justify microsatellite polymorphisms. The C57BL/6J and 129 mouse strains, from which these 29 KO mice were derived, were chosen as the background controls. The results indicated that 10 out of 42 (23.8%) loci showed CMP in some of these mouse strains. Except for the trinucleotide repeat locus of D3Mit22, which had microsatellite CMP in strain number 9, the core sequences of the remaining 41 loci were dinucleotide repeats, and 9 out of 41 (21.95%) showed CMPs among detected mouse strains. However, 11 out of 29 (37.9%) KO mice strains were recognized as having CMPs. The popular dinucleotide motifs in CMP were (TG)(n) (50%, 2/4), followed by (GT)(n) (27.27%, 3/11) and (CA)(n) (23.08%, 3/13). The microsatellite CMP in (CT)(n) and (AG)(n) repeats were 20% (1/5). According to cloning sequencing results, 6 KO mouse strains showed insertions of nucleotides whereas 1 showed a deletion. Furthermore, 2 loci (D13Mit3 and D14Mit102) revealed CMP in 2 strains, and mouse strain number 9 showed CMPs in two loci (D3Mit22 and D13Mit3) simultaneously. Collectively, these results indicated that microsatellite polymorphisms were present in the examined inbred KO mice.  相似文献   

18.
2 congenic strains of mice, B6N.AKN-Ahk and D2N.B6N-Ahb, imported from the USA, were found to be either segregating or fixed for an incorrect allele at a number of biochemical loci. B6N.AKN-Ahk, supposedly congenic with C57BL/6N, had the wrong genotype at 6 out of 12 biochemical loci; D2N.B6N-Ahb, supposedly congenic with DBA/2N, was segregating at 3 out of 9 loci. There was genetic variation in mandible shape within the 2 strains but no abnormal coat colours were found and no hybrid vigour in breeding performance was detected. Analyses in the USA confirmed these results and showed that 2 other congenic strains, C3N.D2N-Ahd and AKN.B6J-Ahb, were also segregating at a number of loci. Some of the alleles found in the C3N.D2N-Ahd mice must be the result of a genetic contamination. The simplest explanation for this breakdown in the backcrossing programme is genetic contamination with other congenic strains or recombinant inbred lines under development in the same laboratory. These findings emphasize the importance of continual genetic monitoring of all genetic stocks at regular intervals and in particular during the development of congenic and recombinant lines.  相似文献   

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