小尾寒羊高繁殖力候选基因ESR的研究

利用PCR—SSCP技术对高繁殖力绵羊品种（小尾寒羊、湖羊、德国肉用美利奴羊）和低繁殖力绵羊品种（多赛特羊、萨福克羊）的雌激素受体（estrogen receptor,ESR）基因第一外显子部分序列进行单核苷酸多态性研究。结果表明：小尾寒羊、湖羊和德国肉用美利奴羊中存在3种基因型（AA、BB、AB）,而在多赛特羊和萨福克羊中只存在两种基因型（AA、AB）。统计结果表明：湖羊、德国肉用美利奴羊、小尾寒羊、萨福克羊和多赛特羊A等位基因频率分别为0．672、0．786、0．846、0．857和0．867,B等位基因频率分别为0．328、0．214、0．154、0．143和0．133。测序结果表明：BB型和AA型相比在外显子1第363位发生1处碱基突变（C→G）。独立性检验表明：小尾寒羊和湖羊之间基因型分布差异极显著（P〈0．01）,湖羊和多赛特羊之间基因型分布差异显著（P〈0．05）,其他各个绵羊品种之间基因型分布差异均不显著。A8基因型和BB基因型小尾寒羊产羔数比AA基因型分别多0．51只（P〈0．05）和0．7只（P〈0．05）。研究结果表明：ESR基因可能是控制小尾寒羊多胎性能的一个主效基因或与之存在紧密的遗传连锁。     

小尾寒羊五个微卫星基因座遗传多态性研究

小尾寒羊是我国优良的地方绵羊品种,具有极高的繁殖力,平均每胎产羔2．6只。利用与绵羊高繁殖力主效基因Fec^B和FecX^1连锁的5个微卫星标记（OarAE101,BM1329,BMS2508,TGLA54t TGLA68)对244小尾寒羊母羊进行了遗传检测。用非变性（中性）聚丙烯酰胺凝胶电泳检测同卫星的PCR扩增产物,计算了5个同卫星基因座的等位基因频率,多态信息含量,基因纯合度和杂合度。在小尾寒羊中检测到BM1329有6个等位基因,片段大小为160－180bp,164bp等位基因频率最高（0．6320）;检测到OarAE101有9个等位基因,片段大小为97－135bp,97bp等位基因频率最高（0．7930）;检测到TGLA54有5个等位基因,片段大小为116－136bp,134bp等位基因频率最高（0．8500）;检测到TGLA68有2个等位基因,片段大小为98－100bp,2个等位基因频率相近,检测到BMS2508有6个等位基因,片段大小为93－115bp,99bp等位基因频率最高（0．4795）。BM1329,OarAE101,TGLA54,TGLA68,BMS2508的多态信息含量／基因纯合度／杂合度分别为0．4481／0．4840．0．5160,0．3516／0．6375／0．3625,0．2528／0．7326／0．2674,0．3733／0．5034／0．4966,0．5809／0．3581／0．6419。可见BMS2508的遗传变异最大,TGLA54的遗传变异最小。这些结果可为小尾寒羊种质特性研究提供分子基础数据。     

小尾寒羊高繁殖力候选基因BMP15和GDF 9的研究

以控制Belclare和Cambridge绵羊高繁殖力的骨形态发生蛋白 15 (bonemorphogeneticprotein 15 ,BMP15 )基因和生长分化因子 9(growthdifferentiationfactor 9,GDF9)基因为候选基因 ,采用PCR RFLP技术检测BMP15基因和GDF9基因在高繁殖力绵羊品种 (小尾寒羊、湖羊 )以及低繁殖力绵羊品种 (多赛特羊、特克塞尔羊、德国肉用美利奴羊 )中的单核苷酸多态性 ,同时研究这两个基因对小尾寒羊高繁殖力的影响。结果表明 :在 5个绵羊品种中都没有检测到GDF9基因的G8突变 (C→T) ,也没有检测到BMP15基因的B4突变 (G→T)。高繁殖力的小尾寒羊在BMP15基因编码序列第 718位碱基处发生了与Belclare绵羊和Cambridge绵羊相同的B2突变 (C→T) ,而其余 4个绵羊品种则没有发生这种突变。对于BMP15基因的B2突变 ,在小尾寒羊中检测到AA、AB两种基因型 ,A等位基因频率为 0 734,B等位基因频率为 0 2 6 6。小尾寒羊与其余 4个绵羊品种间B2突变基因型分布差异极显著 (P <0 0 0 1)。突变杂合基因型 (AB)小尾寒羊平均产羔数比野生纯合基因型 (AA)多 0 6 2只 (P <0 0 1)。研究结果表明 ,BMP15B2突变对小尾寒羊高繁殖力影响作用十分明显 ,同时排除了GDF9G8突变和BMP15B4突变影响小尾寒羊高繁殖力的可能性     

泌乳素及其受体的研究进展

泌乳素(PRL)又名催乳素,是由腺垂体及一些垂体外器官如乳腺、胸腺、脾脏等合成的一种多肽类激素,以内分泌、自分泌、旁分泌的形式发挥作用,其广泛参与机体生长发育、物质代谢、性腺功能调节、应激反应、免疫调节等。泌乳素通过与其受体(PRL receptor,PRLR)在靶细胞的细胞膜表面结合,激活下游的信号转导通路,发挥其生物学作用。由于泌乳素在人体内复杂的生物学效应,泌乳素及其受体又与乳腺癌、泌乳素瘤等多种疾病的发生发展及其预后密切相关。本文就泌乳素发挥效应时对其受体的激活、受体激活后的信号转导机制以及泌乳素同相关疾病的联系进行了综述,相信泌乳素及其受体的研究将为这些疾病的治疗提供重要的方向。     

Association Between PCR-SSCP of Bone Morphogenetic Protein 15 Gene and Prolificacy in Jining Grey Goats

The Jining Grey is a prolific local goat breed in P.R. China. Bone morphogenetic protein 15 (BMP15) gene that controls high fecundity of Inverdale, Hanna, Lacaune, Belclare, Cambridge, and Small Tailed Han ewes was studied as a candidate gene for the prolificacy of Jining Grey goats. According to the sequence of ovine BMP15 gene, six pairs of primers were designed to detect single nucleotide polymorphisms in exon 1 and exon 2 of the BMP15 gene in both high fecundity breed (Jining Grey goats) and low fecundity breeds (Boer, Liaoning Cashmere, and Inner Mongolia Cashmere goats) by single strand conformation polymorphism (SSCP). Two pairs of primers (F1/R1 and F2/R2) were used to amplify the exon 1. Four pairs of primers (F3/R3, F4/R4, F5/R5, and F6/R6) were used to amplify the exon 2. Only the products amplified by primer F5/R5 displayed polymorphism. Results indicated that two genotypes (AA and AB) were detected in prolific Jining Grey goats and only one genotype (AA) was detected in low fecundity goat breeds. In Jining Grey goats frequencies of genotypes AA and AB were 0.10 and 0.90, respectively. Sequencing revealed two point mutations (G963A and G1050C) of BMP15 gene in the AB genotype in comparison to the AA genotype. In Jining Grey goats the heterozygous AB does had 1.13 (p < 0.01) kids more than the homozygous AA does. These results preliminarily showed that the BMP15 gene is either a major gene that influences the prolificacy of Jining Grey goats or a molecular genetic marker in close linkage with such a gene.     

乐至黑山羊PRLR基因外显子10多态性与产羔数的关系研究

设计2对特异性引物对乐至黑山羊PRLR基因第10外显子进行了PCR-SSCP检测,并研究该基因与产子性能的相关性。结果表明,P1引物扩增片段不存在多态性;P2引物扩增片段存在多态性,表现为AA,AB,AD和CD 4种基因型,测序结果表明,4种基因型都在该片段第89、94、146和157位存在C→T、A→C、C→G、G→C的突变;此外AA型还在61位发生C→T的突变;AD型还在175位发生A→G的突变;CD型还在24位发生T→C的突变,96位发生C→T的突变,通过统计分析发现AD型平均产羔数优于其他3种基因型,并且与AB型差异达到显著水平(P<0.05)。因此认为PRLR基因对于乐至黑山羊产子性能有一定的影响。     

甘肃肉羊新品种选育群GDF9基因外显子2多态性及其与产羔性状关联分析

根据GenBank发布的绵羊GDF9基因外显子2的序列设计4对引物,采用PCR-SSCP技术分析GDF9基因外显子2在甘肃内羊新品种选育群羊中的单核苷酸多态性,并与产羔性状进行关联分析.结果表明,GDF9基因的扩增片段在所检测的新品种群羊中存在PCR-SSCP多态性,检测到3种基因型(AA、AB和BB),而在32只无角陶赛特母羊群中只检测到AA和AB基因型.测序结果显示,GDF9基因编码区第978位碱基发生A→G突变,但没有导致氨基酸的改变;第994位碱基发生G→A突变,导致Ⅴ变成Ⅰ(缬氨酸→异亮氨酸).新品种选育群羊产羔数的最小二乘均值关系为AB＞ AA＞ BB,统计分析结果初步表明3种基因型之间差异不显著(P＞0.05).故该区域可能不是影响新品种群羊繁殖力的功能结构区城.     

催乳素受体基因的研究进展

本文介绍催乳素受体的结构,催乳素受体基因的发育性表达及作用,催乳素受体基因的作用机理与分子调控,催乳素受体基因的定位以及其与繁殖性状的关系等。提示催乳素受体基因可作为繁殖性状的一个候选基因。 Abstract:This review introduced the structure of prolactin receptor,the developmental expression and function,action　mechanism and molecular regulation,mapping of prolactin receptor gene and its relationship with reproductive traits.These revealed that prolactin receptor gene could be used as a candidate gene for reproductive traits.     

BMPR-IB和BMP15基因作为小尾寒羊多胎性能候选基因的研究

以控制BooroolaMerino羊多胎性能的BMPR IB基因 ,以及影响Invedale和Hanna羊排卵数的BMP15基因作为候选基因 ,从分子水平上对小尾寒羊的多胎机制进行研究 ,分析突变位点的特性 ,并通过大规模的群体检测统计推断其遗传效应。实验结果表明 :多胎品种小尾寒羊在BMPR IB基因的相应位置上发生了与BooroolaMerino羊相同的突变 (A74 6G) ,该基因的BB基因型在小尾寒羊群体内为优势基因型 ,且小尾寒羊初产和经产母羊的BB基因型比 ++基因型分别多产 0 97羔 (P <0 0 5 )和 1 5羔 (P <0 0 1) ,推测BMPR IB基因与控制小尾寒羊多胎性能的主效基因存在紧密的遗传连锁。而BMP15基因在小尾寒羊中不存在V31D或Q2 3Ter突变 ,说明小尾寒羊的多胎遗传机制与Romney羊不同 ,因此排除了BMP15突变影响小尾寒羊排卵数的可能性。     

小尾寒羊4个微卫星座位的克隆及序列分析

小尾寒羊是我国优良的地方绵羊品种 ,具有极高的繁殖力 ,平均每胎产羔 2 6只。利用与Booroola绵羊高繁殖力主效基因 FecB连锁的 4个微卫星座位 OarAE10 1、OarHH35、BM14 3和BMS2 5 0 8对小尾寒羊、多赛特羊、多赛特公羊×小尾寒羊母羊杂一代羔羊 3个绵羊群体 15 9只绵羊进行了遗传检测 ,证实了微卫星DNA的共显性遗传特性。用非变性 (中性 )聚丙烯酰胺凝胶电泳检测微卫星的PCR扩增产物。对小尾寒羊 4个微卫星座位 6个克隆的PCR扩增片段测序获得的序列已被GenBank接受 ,登录号分别为AF394 4 4 5、AF394 4 4 6、AF394 4 4 7、AF394 4 4 8、AF394 4 4 9、AF394 4 5 0。本研究中小尾寒羊微卫星OarAE10 1的测序结果与GenBank登录的绵羊OarAE10 1序列的同源性为 98% ,小尾寒羊微卫星OarHH35的测序结果与GenBank登录的绵羊OarHH35序列的同源性为 99% ,小尾寒羊微卫星BM14 3的测序结果与GenBank登录的牛BM14 3序列的同源性为 95 % ,小尾寒羊微卫星BMS2 5 0 8的测序结果与GenBank登录的牛BMS2 5 0 8序列的同源性为 95 %。测得的小尾寒羊微卫星OarAE10 1、OarHH35、BM14 3和BMS2 5 0 8均为完全的微卫星 (TG) n。这些结果可为小尾寒羊种质特性研究提供分子基础数据     

乳房肥大乳腺组织中泌乳素及其受体的表达

目的:研究泌乳素(PRL)及其受体(PRLR)在乳房肥大和正常体积乳房中的表达情况,探讨乳腺组织中PRL、PRLR的表达与乳房肥大的相关性,为乳房肥大的治疗提供方向。方法:收集2013年1月~2013年4月第四军医大学西京医院26例乳房肥大患者和16例因单纯乳房下垂行乳房悬吊术患者的乳腺组织,采用免疫组织化学法检测乳腺组织标本中PRL和PRLR的表达。结果:PRL在乳房肥大组和正常体积乳房组乳腺组织中的阳性细胞率分别为88.46℅和56.25℅,两组比较差异有统计学意义(P0.05),且两组的PRL阳性的细胞面积、平均光密度值和累积光密度值均有统计学差异(P0.05)。乳房肥大组和正常体积乳房组乳腺组织中PRLR的阳性细胞率分别为76.92℅和75.00℅,两组比较无明显的统计学差异(P0.05),且两组间的PRLR阳性的细胞面积、平均光密度值、累积光密度值均无明显的统计学差异(P0.05)。结论:乳房肥大的发生可能与乳腺组织中泌乳素的表达升高有关,而与乳腺组织中泌乳素受体的表达无关。     

高原型藏羊和小尾寒羊睾丸小叶及附睾微动脉的解剖学特征

分别从青海和甘肃采集高原型藏羊(Ovis aries)和小尾寒羊睾丸各20枚,用血管铸型技术和扫描电镜方法,研究两品种绵羊睾丸小叶及附睾微动脉的超微形态特征。结果显示,两品种绵羊的睾丸小叶及附睾微动脉走形呈一定程度的弯曲,其中睾丸小叶内离心动脉、离心小动脉及向心小动脉均呈"树枝"状分布。研究发现,与低海拔地区的小尾寒羊相比,高原型藏羊睾丸的绳结状动脉具有更密集的螺旋状排布,小动脉分支也较多,并且向心动脉、绳结状动脉、离心动脉、附睾头微动脉的管径也较粗。此外,高原型藏羊睾丸小叶和附睾头微动脉表面的"梭形"压痕较浅,而小尾寒羊的则较深;高原型藏羊睾丸小叶毛细血管前微动脉的表面缢痕较多且密集,而小尾寒羊的则相对少而稀疏。研究认为,高原型藏羊睾丸小叶及附睾微动脉的超微形态特征,有利于血管的收缩、睾丸供血及高原环境下精子的成熟,是睾丸对高原环境的适应性特征。     

Ex-FABP 作为鸡腹脂性状主要候选基因的研究

细胞外脂肪酸结合蛋白 (extracellular fatty acid-binding protein, Ex-FABP) 基因是脂肪酸结合蛋白 (fatty acid-binding protein, FABP) 家族的另一成员,参与鸡的脂肪酸、肌纤维、骨骼等调控过程 . 利用 PCR-SSCP (single strand conformation polymorphism) 和 DNA 测序的方法,对不同品种的杂交鸡进行了 Ex-FABP 基因 5′调控区部分序列的多态性分析,发现了 3 个单核苷酸多态性 (single nucleotide polymorphisms, SNPs) 位点 . 其中,此片段中的碱基 C (－1000) 的插入和碱基 T → C (－1011) 的突变,导致此处比野生型基因少了 1 个 cap ,多了 1 个 Nkx-2 、 1 个 AhR/Ar 和 2 个 CF1 等转录因子结合位点的产生 . 利用 SAS 软件对 Ex-FABP 基因 5′调控区的 SNPs 与屠体性状的最小二乘分析,发现基因型 BB (突变型) 与腹脂重存在极显著相关 (P<0.01). 研究结果表明,细胞外脂肪酸结合蛋白 (Ex-FABP) 基因是影响脂肪沉积、控制腹脂性状的主要候选基因 .     

上海地区汉族人5-HT2a受体基因T102C多态性的基因频率分布

为了揭示中国汉族人5-HT2a受体基因T102C多态性基因频率的分布,我们随机抽取了226例汉族健康人作研究,用限制性片段长度多态性(RFLPs)技术测定研究对象的基因型和等位基因。结果发现汉族正常人5-HT2a受体基因T102C多态性基因型频率依次为:A1/A2=0.5044,A1/A1=0.2965,A2/A2 =0.1991,两种等位基因频率依次为:A1=0.5487,A2=0.4513,杂合度H=0.50 44、期望杂合度h=0.4953,多态信息量PIC=0.3726,表明T102C多态性具有合适信息,对疾病的关联研究,法医学鉴定有一定的价值。 Abstract:To investigate the distribution about genotype and allele frequencies of T102C polymorphism in the 5-HT2a receptor gene Chinese Han population,the genotypes and alleles of 226 healthy person were examined with Restriction Fragment Length Polymorphisms(RFLPs)technique.The genotype frequencies are as follows:A1/A2=0.5044,A1/A1=0.2965,A2/A2=0.1991,respectively,and the allele frequencies are as follows:A1=0.5487,A2=0.4513,respectively.The heterozygosity(H)is 0.5044,the expected heterozygosity(h)is 0.4953,and the Polymorphism Information Content(PIC)is 0.3726.Our findings suggest that the T102C polymorphism in 5-HT2a receptor gene may have suitable information to be used for association study or forensic identification.     

Cryopreservation and multipotential characteristics evaluation of a novel type of mesenchymal stem cells derived from Small Tailed Han Sheep fetal lung tissue

Lung mesenchymal stem cells (L-MSCs) characterized by plasticity, reduced relative immune privilege and high anti-fibrosis characteristics play the crucial role in lung tissue regenerative processes. However, up to date, the multi-differentiation potentials and application values of L-MSCs are still uncertain. In the current study, the Small Tailed Han Sheep embryo L-MSCs line from 12 samples, stocking 124 cryogenically-preserved vials, was successfully established by using primary culture and cell cryopreservation techniques. Isolated L-MSCs were morphologically consistent with fibroblasts, could be passaged for at least 18 passages and more than 91.8% of cells were diploid (2n = 54) analyze by G-banding. The majority of cells were in the G0/G1 phase (70.5–91.2%), and the growth curves were all typically sigmoidal. Moreover, L-MSCs were found to express pluripotent genes Oct4, Nanog and MSCs-associated genes β-integrin, CD29, CD44, CD71, CD73 and CD90, while the expressions of hematopoietic cell markers CD34 and CD45 were negative. In addtion, the L-MSCs could be differentiated into cells of three layers with induction medium in vitro, which confirmed their multilineage differentiation potential. The secretion of urea and ALB showed the differentiated hepatocytes still possessed the detoxification function. These results indicated that the isolated L-MSCs displayed typical characteristics of mesenchymal stem cells and that the culture conditions were suitable for their maintenance of stemness and their proliferation in vitro.     

GDF9 as a candidate gene for prolificacy of Small Tail Han sheep

Growth differentiation factor 9 (GDF9) which controls the fecundity of Belclare, Cambridge, Santa Ines, Moghani, Ghezel and Thoka ewes was studied as a candidate gene for the prolificacy of Small Tail Han sheep. According to the sequence of ovine GDF9 gene, six pairs of primers were designed to detect single nucleotide polymorphisms of two exons of GDF9 gene in both high fecundity breed (Small Tail Han sheep) and low fecundity breed (Dorset sheep) by polymerase chain reaction-single strand conformation polymorphism (PCR-SSCP). Only the products amplified by primers 2-1 and 2-2 displayed polymorphisms. For primer 2-1, three genotypes (AA, AB and BB) were detected in both sheep breeds. Sequencing revealed one silent mutation (G477A) in exon 2 of GDF9 gene in the BB genotype in comparison with the AA, which was known as G3 mutation of GDF9 gene in Belclare and Cambridge ewes. The relationship of least squares means for litter size was AA?>?AB?>?BB in Small Tail Han sheep (P?>?0.05). For primer 2-2, two genotypes (CC and CD) were detected in both sheep breeds. Sequencing revealed one novel single nucleotide mutation (G729T) in exon 2 of GDF9 gene in the CD genotype in comparison with the CC, which resulted in an amino acid change (Gln243His). The ewes with mutation heterozygous genotype CD had 0.77 (P?相似文献   

绵羊产羔性状主效基因检测研究

以绵羊BMP15基因和BMPR-IB基因为候选基因,以湖羊、中国美利奴单胎品系、中国美利奴肉用和毛用多胎品系为研究对象,采用PCR-RFLP方法对候选基因进行单核苷酸多态性（SNP）位点检测和基因型分析,同时研究基因对绵羊产羔数的影响。对BMP15基因进行SNP检测,结果未发现多态性位点;对BMPR-IB基因进行多态性检测,结果发现了一个A746 G SNP位点。依据A746 G SNP位点进行基因型分析,结果在各品种（系）羊中发现了3种基因型,即BB、B+和++。等位基因型频率在各品种（系）间差异极显著（P<0.001）,在湖羊中以BB基因型为主,在中国美利奴单胎品系中以++基因型为主, 而在中国美利奴肉用和毛用多胎品系中以B+基因型为主。BMPR-IB A746G位点的变异明显影响绵羊的产羔数,与++基因型母羊相比, BB和B+基因型母羊产羔数明显较多。研究结果同时表明,利用BMPR-IB基因型可以很好的预测母羊的产羔数。研究获得的这些结果强烈表明BMPR-IB为影响绵羊的产羔数的主效基因,可以用于对绵羊产羔数的选择。Abstract: The current study was designed to detect SNPs within BMP15 and BMPR-IB gene and investigate the effect of the genes on sheep litter size. Four sheep lines, HU-Yang, Chinese M erino monotocous, Chinese Merino multiparous for wool production and Chinese Merino multiparous for mutton production, were used in this study. Litter sizes were recorded for each ewe in the four lines. Primers for BMP15 and BMPR-IB gene were designed from database sheep sequence and polymorphisms were detected by PCR-RFLP method. The results showed that there was no polymorphism with BMP15 gene among the four lines, and there was an A / G SNP with BMPR-IB gene at base 746 among the four lines. Three types of genotype (BB, B+ and ++), based on A / G locus, were found within each line. The frequencies of genotypes were significantly different among the lines (P<0.001), with BB genotype primarily existing in HU-Yang, ++ genotype in Chinese Merino monotocous line, and B+ genotype in Chinnese Merino multiparous lines. The A / G mutation influence significantly the sheep litter sizes, and the BB and B+ ewes had significant higher litter sizes than ++ ewes. The results of present study showed simultaneously that the genotype of BMPR-IB was a perfect predictor of the sheep litter sizes. These results intensively indicated that BMPR-IB is a major gene to affect litter size in sheep, and could be used as the molecular genetic marker to select litter size in sheep.     

催乳素受体基因与羊驼繁殖性能关系的初探

通过氯仿/异戊醇法制备羊驼血液基因组DNA,采用PCR方法首次扩增出羊驼催乳素受体基因(prolactin receptor gene,PRLR)exon8-exon9序列(GenBank登录号为DQ198164),该片段长度为622bp。通过NCBI blast(http://www.ncbi.nlm.nih.gov/BLAST/)比较,结果表明:该序列包括exon8的82bp、intron8全序列472bp和exon9的68bp。同源性比较发现,羊驼PRLR基因exon8和exon9核苷酸序列与其它哺乳动物的相应区域的同源性特高,均≥92%;同时还发现羊驼exon8引物后第19个碱基为G,而其它哺乳动物(猪除外)均为A,猪则是在羊驼exon8引物后的第34个碱基处由G变为A,通过推导氨基酸序列分析发现,这种单碱基的突变使得羊驼与其它哺乳动物相比,该处的氨基酸由亮氨酸取代了异亮氨酸;在羊驼exon9引物前第22个碱基处也发生了A-G碱基替换现象,但这个碱基的突变发生在密码子的第3个碱基上,编码的氨基酸均为脯氨酸。在这些动物中只有羊驼为单胎动物,羊驼exon8核苷酸序列中A-G的碱基替换并引起编码氨基酸序列发生改变是否与羊驼繁殖性能有关还有待进一步研究。     

四引物扩增受阻突变体系PCR快速测定绵羊 BMPR-IB基因型方法的建立

四引物ARMS PCR是检测SNP有效、快速、简便的方法.绵羊BMPR-lB基因是控制Booroola绵羊多胎性状的主效基因,此研究目的在于建立一种对BMPR-IB基因四引物ARMS PCR检测方法.根据四引物ARMS PCR技术原理,在绵羊BMPR-IB基因突变位点(A746G)设计一对特异性引物,并在突变点两侧设计一对参照引物,用来扩增含有突变点的DNA片段,可在一步PCR反应中根据电泳图谱准确判断绵羊个体的BMPR-IB基因型,对比PCR-RFLP检测结果表明,所建立的方法简单,操作简便,大大提高了检测效率.