Effect of in ovo zinc injection on the embryonic development, tissue zinc contents, antioxidation, and related gene expressions of broiler breeder eggs

Two experiments were conducted to investigate the effect of in ovo zinc （Zn） injection on the embryonic development, tissue Zn contents, antioxidation and related gene expressions of fertilized eggs of Arbor Acres broiler breeders. Experiment 1 was conducted to determine an optimal embryonic age for early in ovo injection. A total of 720 fertilized eggs with similar weights were randomly allotted to 4 treatments with 6 replicates per treatment and 30 eggs per replicate in a completely randomized design. The eggs were injected with 0.1 mL sterilized water at 3, 6 and 9 embryonic days of incubation （E3, E6 and E9） or non-injection （the control）, respectively. The results from experiment 1 showed that E3 and E6 injections increased （P〈0.05） the embryonic mortalities, and decreased （P〈0.05） hatchabilities compared to the non-injected control, but no differences （P〉0.05） between E9 injection and the non-injected control were observed in either embryonic mortality or hatchability. The findings suggest that the E9 is the optimal embryonic age for early in ovo injection. In experiment 2, a total of 672 fertilized eggs with similar weights were randomly allocated to 7 treatments with 6 replicates per treatment and 16 eggs per replicate in a completely randomized design. The eggs were injected with 0 （the negative control）, 50, 100, 150, 200, or 250 μg Zn/egg as reagent grade ZnSO4.7H20 in a 0.1-mL solution, or non-injection （the positive control）, respectively at E9-10. The results from the experiment 2 demonstrated that no differences （P〉0.05） among 50 and 100 μg Zn/egg groups and the negative control were observed in the embryonic mortality and hatchability, however, the injection of 200 μg Zn/egg increased （P〈0.05） the embryonic mortality, and injections of 150 and 200 μg Zn/egg decreased （P〈0.05） hatchabilities compared with the controls. The embryonic tibia Zn contents at E20 were increased （P〈0.05） by injections of 150, 200 and 250μg Zn/egg. Zinc injection did not affect （P〉0.05） malonaldehyde （MDA） contents, copper- and Zn- containing superoxide dismutase （CuZnSOD） activities and mRNA expression levels in the liver and heart of chick embryos at E15 and E20. Compared with the negative control, injections of 50, 150 and 200 μg Zn/egg up-regulated （P〈0.05） themetallothionein （MT） mRNA expression levels in the embryonic liver at E20. These results indicated that in ovo Zn injections increased Zn contents in the embryonic tibia and MT mRNA expression levels in the embryonic liver at E20, however, injections of 150-200 μg Zn/egg were harmful to the embryonic development.

Effects of NPY Gene on Total Number of Eggs at 300 Days of Age in Donglan Black-bone Chicken

In this study, PCR-RFLP technique was employed to detect the genetic polymorphism of NPY gene and analyze the effects of various genotypes on the total number of eggs at 300 days of age in 135 Donglan black-bone chicken. According to the results, there were three genotypes （AA, AB and BB） of NPYgene in Donglan black-bone chicken group. Different genotypes exhibited significant effects （P 〈 0. 05 ） on the total number of eggs at 300 days of age. The total number of eggs at 300 days of age of AA genotype was significantly higher than that of BB genotype （P 〈 0. 05）. Therefore, the polymorphic site of NPY gene could be used as a candidate molecular marker that affects egg laying in Donglan black-bone chicken.

A significant quantitative trait locus on chromosome Z and its impact on egg production traits in seven maternal lines of meat-type chicken

Background:Egg production is economically important in the meat-type chicken industry.To better understand the molecular genetic mechanism of egg production in meat-type chicken,genetic parameter estimation,genome-wide association analyses combined with meta-analyses,Bayesian analyses,and selective sweep analyses were performed to screen single nucleotide polymorphisms(SNPs)and other genetic loci that were significantly associated with egg number traits in 11,279 chickens from seven material lines.Results:Yellow-feathered meat-type chickens laid 115 eggs at 43 weeks of age and white-feathered chickens laid 143 eggs at 60 weeks of age,with heritability ranging from 0.034–0.258.Based on meta-analyses and selective sweep analyses,one region(10.81–13.05 Mb)on chromosome Z was associated with egg number in all lines.Further analyses using the W2 line was also associated with the same region,and 29 SNPs were identified that significantly affected estimation of breeding value of egg numbers.The 29 SNPs were identified as having a significant effect on the egg number EBV in 3194 birds in line W2.There are 36 genes in the region,with glial cell derived neurotrophic factor,DAB adaptor protein 2,protein kinase AMP-activated catalytic subunit alpha 1,NAD kinase 2,mitochondrial,WD repeat domain 70,leukemia inhibitory factor receptor alpha,complement C6,and complement C7 identified as being potentially affecting to egg number.In addition,three SNPs(rs318154184,rs13769886,and rs313325646)associated with egg number were located on or near the prolactin receptor gene.Conclusion:Our study used genomic information from different chicken lines and populations to identify a genomic region(spanning 2.24 Mb)associated with egg number.Nine genes and 29 SNPs were identified as the most likely candidate genes and variations for egg production.These results contribute to the identification of candidate genes and variants for egg traits in poultry.

Correlation between DRD2 Gene Polymorphism and Early Egg Production Performance of Libo Yaoshan Chicken

To improve egg production performance of local chicken breed in Guizhou Province, Libo Yaoshan chicken, with dopamine receptor 2 （ DRD2 ） as one of the candidate genes, we detected its genetic variation in 196 Libe Yaoshan hens using PCR-SSCP （single-strand conformation polymorphism） and sequencing method, and analyzed the correlation between genetic variation and egg production traits. The results showed that TT and TG genotypes in mRNA SNlX）62 （C→T） loci of the DRD2 gene had extremely significant difference in egg production at 38 weeks age （P 〈0.01 ）, and significant difference in egg weight at 300 days age （P 〈0.05 ）. The single nucleotide polymorphisms （SNPs） mutation induced synonymous mutation of the 312th amino acids （leucine） in DRD2 protein, from L （CTG） to L （TI＇G）. The mRNA SNP962 （C→T） loci had a larger genetic effect on egg production at 38 weeks age, and could be used as a molecular marker in early breeding of Libo Yaoshan chicken.

高邮鸭Akt1基因克隆及生物信息学分析

Akt1是丝氨酸/苏氨酸蛋白激酶家族基因,通过响应生长因子刺激磷酸化一系列下游底物来调节许多过程,包括代谢、增殖、细胞存活、生长和血管生成等。实验室前期对全转录组差异分析获得了与高邮鸭双黄蛋率显著相关的候选关键基因Akt1,并且Akt1显著富集于差异表达信号通路——PI3K-AKT信号通路。为了对高邮鸭双黄蛋候选基因Akt1进行系统的功能研究,本研究通过PCR技术克隆高邮鸭卵巢组织Akt1全长,构建了Akt1-EGFP融合表达载体,结合生物信息学技术对AKT1蛋白的理化性质进行系统分析。结果:AKT1为种间保守型非分泌蛋白,表达于质膜,具有丰富的丝氨酸和苏氨酸磷酸化位点,可与10种蛋白(TSC1、MAPK1、PIK3R1、PIK3CA、TSC2、CDKN1A、IKBKB、PIK3CD、PDPK1和ILK)发生互相作用。研究结果为揭示Akt1基因编码的蛋白在调控高邮鸭双黄蛋形成过程中的功能和分子机制提供理论基础。

SLCO1C1和SLCO4C1基因与绿壳蛋鸡不同产蛋期壳色相关性研究

为探究SLCO家族基因与绿壳蛋壳色的关系,试验以产绿壳蛋母鸡为试验样本,分别收集产蛋前期(150日龄)和产蛋后期(500日龄)的鸡蛋、心脏、肝脏、脾脏、肌肉、卵巢、壳腺组织和血样样品,采用色差仪测定壳色数值;ELISA方法检测血清中血红素加氧酶1(HO-1)的含量;利用荧光定量PCR测定HO-1和SLCO家族基因的表达。结果显示:产蛋前期蛋壳L*值极显著低于产蛋后期(P<0.01),而b*值极显著高于产蛋后期(P<0.01);产蛋前期血清中HO-1含量和壳腺中HO-1表达量极显著高于产蛋后期(P<0.01);SLCO1C1和SLCO4C1在壳腺中特异性表达,SLCO1A2在肝脏中特异性表达;产蛋前期SLCO1C1和SLCO4C1 mRNA表达量显著高于产蛋后期(P<0.05)。结果表明HO-1基因表达与酶活性下降造成绿壳蛋鸡壳色变浅,SLCO1C1和SLCO4C1可能是胆绿素合成和转运的重要基因。

鸡蛋蛋壳颜色的形成及其影响因素

禽蛋是家禽的主要产品之一,蛋壳的颜色影响其销售,生产者与研究人员一直关注如何选择与调控家禽的蛋壳颜色。家禽蛋壳中的主要色素大致分为三种,即原卟啉Ⅸ、胆绿素Ⅸ和胆绿素锌螯合物。文章对蛋壳颜色的形成、影响因素和关联基因等方面进行综述,以促进家禽蛋壳颜色的研究。

仰口线虫PCR检测方法的建立及应用

为特异性检测羊感染仰口线虫的情况,基于仰口线虫ITS基因序列设计特异性引物,进行退火温度及反应条件的优化,建立其属特异性PCR检测方法。应用该方法对仰口线虫、食道口线虫、毛尾线虫、捻转血矛线虫、细颈线虫、奥斯特线虫、夏伯特线虫、筒线虫、毛圆线虫的DNA样本进行扩增,仅能特异性扩增出仰口线虫的目的条带;该方法成功从仰口线虫中扩增出约500 bp的特异性片段,最低检测浓度为3.6×10^(3)copies/μL;该PCR检测方法对临床奶山羊粪便样品的检测结果显示,羊粪便样品中仰口线虫卵的阳性率为10%,且与显微镜镜检所得的结果一致。结果表明,建立的仰口线虫PCR检测方法敏感性较高且特异性良好,可以应用于临床羊粪便样品中仰口线虫的虫卵检测,为羊仰口线虫病的诊断与防治提供了一种技术支持。

生长激素基因SNPs与康乐黄鸡产蛋性状的关联分析

为探索生长激素(Growth hormone,GH)基因部分序列单核苷酸多态性(Single nu⁃cleotide polymorphism,SNP)位点与康乐黄鸡母鸡产蛋性状的相关性,寻找地方鸡种产蛋性状选育的分子标记,试验选取294只康乐黄鸡母鸡为研究材料,测量并记录3个产蛋性状指标,包括开产日龄、初产体重和182日龄产蛋数。采用PCR直接测序法筛选GH基因内含子1区域SNPs,利用SAS分析产蛋性状关联的SNPs。结果显示:共发现30个SNP位点,其中共有5个SNP位点与康乐黄鸡母鸡产蛋性状显著关联,其中位于内含子1区域的位点T1270451C与康乐黄鸡母鸡182日龄产蛋数,位点C1271148T与开产日龄、初产体重,位点A1271168G与开产日龄,位点G1271198A与初产体重均显著相关,位于内含子2区域的位点T1270070A与初产体重显著相关。研究表明,GH基因内含子1区域的4个位点T1270451C、C1271148T、A1271168G、G1271198A,内含子2区域T1270070A位点可作为康乐黄鸡产蛋性状选育的候选分子标记。

沟眶象味觉受体基因EscrGR8对雌成虫繁殖力的影响

【目的】分析和阐明沟眶象Eucryptorrhynchus scrobiculatus味觉受体基因EscrGR8的分子特性和功能,揭示其调节雌成虫繁殖力的作用。【方法】基于沟眶象触角转录组数据库,采用RACE克隆EscrGR8的cDNA全长序列;利用qRT-PCR检测EscrGR8在沟眶象不同发育阶段(卵、1-6龄幼虫、蛹、雌成虫和雄成虫)和雌雄成虫组织(去除触角和喙的头、触角、口器、中肠、前足、睾丸、卵巢、雄虫交配器和雌虫产卵器)中的表达量。显微注射雌成虫dsRNA后0,6,12,24,36,48和72 h时利用qRT-PCR检测RNAi后EscrGR8的表达量。检测显微注射dsEscrGR8后1-5 d和6-11 d时沟眶象雌成虫在不同土壤含水量(0~10%,11%~20%,21%~40%,41%~60%,61%~80%和81%~100%)条件下的产卵选择率、总产卵数量和所产卵的孵化率,研究抑制EscrGR8表达对雌成虫产卵选择性和繁殖力的影响。【结果】成功克隆了沟眶象EscrGR8(GenBank登录号:OR836580)的cDNA全长序列,开放阅读框(ORF)长1251 bp,编码了416个氨基酸,具有6个跨膜结构域。多序列比对和系统发育进化分析结果表明,EscrGR8与其他昆虫的GR的氨基酸序列同源性普遍较低,其中与棉铃象甲Anthonomus grandis的AgraGR64f氨基酸序列一致性为30.96%。qRT-PCR检测结果表明,EscrGR8在沟眶象不同发育阶段和成虫组织中的表达量具有显著差异,EscrGR8在雌成虫中的表达量最高,在卵中的表达量最低;EscrGR8在雌成虫卵巢中特异性高表达。显微注射dsEscrGR8不仅在一定时间内显著降低EscrGR8的表达量,并且对雌成虫的产卵选择性具有显著影响。显微注射dsEscrGR8后1-5 d时沟眶象雌成虫在含水量21%~40%土壤条件下的产卵选择率和所产卵的孵化率与显微注射dsGFP的对照组相比分别显著降低了24.66%和15.83%;在含水量81%~100%土壤条件下的产卵选择率与显微注射dsGFP的对照组相比显著增加了28.39%,雌成虫所产卵几乎不孵化。【结论】本研究证实了味觉受体基因EscrGR8对沟眶象雌成虫产卵选择和繁殖力的影响,有助于理解昆虫味觉受体基因的多样性和功能特异性。

鸡慢羽基因型在不同品种中多态性及其与产蛋性状相关性研究

研究旨在丰富慢羽基因型的分子标记并探究慢羽基因型与产蛋量的相关关系。试验基于2个慢羽母鸡群体京红1号父母代种鸡母本和欣华鸡母本鉴定慢羽基因型的种类,采用PCR扩增方法检测个体中融合基因dPRLR-dSPEF2和内源性逆转录病毒ev21基因的插入情况。结果显示:在两个慢羽母鸡群体中存在6种不同的慢羽基因型,当个体存在ev21基因(OR)或融合基因dPRLR-dSPEF2中的任意一种或两种时均表现为慢羽,当无ev21基因(UR)且融合基因dPRLR-dSPEF2也不存在时,表现为快羽;11个其他品种快慢羽基因型频率统计发现不同的品种快慢羽基因型频率存在差异。个体中携带融合基因dPRLR-dSPEF2时,其产蛋量会显著高于不携带者(P<0.05);与仅携带ev21基因(OR突变)的个体相比,同时携带ev21基因(OR突变)和正常UR区域的产蛋量有显著升高(P<0.05)。研究表明,ev21插入和融合基因并非鸡快慢羽的唯一关联突变,且京红1号父母代群体中慢羽基因型间存在显著的产蛋量差异。

基于基因组重测序筛选籽鹅产蛋性状候选基因

为筛选参与调控籽鹅产蛋性状的关键基因,依据产蛋记录选取300日龄高低产籽鹅各30只,采血并提取基因组DNA,基于基因组重测序结果筛选差异SNPs并注释基因,应用群体分化指数(Fst)选择信号分析后,进行GO功能和KEGG通路富集分析,筛选与籽鹅产蛋性状相关候选基因。结果表明:2~15周高产籽鹅产蛋率显著高于低产籽鹅(P<0.01);重测序共生成数据1556.48 Gb(n=60),平均深度为21.62倍,平均覆盖率为98.78%;高、低产籽鹅分别筛选到12187636和12291795个SNPs,变异主要位于内含子和非编码区;Fst选择信号分析共筛选出829个候选基因,GO功能和KEGG通路富集分析筛选出MAPK9、TGFB2和SGPL1基因与产蛋性能相关。说明MAPK9、TGFB2和SGPL1可作为籽鹅产蛋性状的候选基因。

Interaction mechanism of egg white-derived ACE inhibitory peptide TNGIIR with ACE and its effect on the expression of ACE and AT1 receptor

The egg white-derived hexapeptide TNGIIR inhibits angiotensin-converting enzyme(ACE)activity in vitro.In this work,molecular docking revealed that TNGIIR established hydrogen bonds with the S1(Ala 354),S2(Gln 281,His 513,Tyr 520 and Lys 511)and S1(Glu 162)pockets of ACE.In addition,the potential antihypertensive effect of the oral administration of TNGIIR in spontaneously hypertensive rats(SHR)was investigated,as was the effect of this peptide on the mRNA expression of ACE and angiotensin type 1(AT1)and type 2(AT2)receptors in renal tissue.The oral administration of TNGIIR(2,10 and 50 mg/kg)for up to four weeks did not reduce the blood pressure of SHR,in contrast to captopril(10 mg/kg,orally),but attenuated the mRNA expression of ACE and AT1 receptor(as did captopril).In contrast,both TNGIIR and captopril enhanced the expression of AT2 receptor mRNA.There was no change in the circulating concentration of angiotensin I,but a slight decrease(about 10%)was seen in the concentration of circulating angiotensin II with TNGIIR and captopril.

The mechanism of sperm-egg interaction and the involvement of IZUMO1 in fusion

An average human ejaculate contains over 100 million sperm, but only a few succeed in accomplishing the journey to an egg by migration through the female reproductive tract. Among these few sperm, only one participates in fertilization. There might be an ingenious molecular mechanism to ensure that the very best sperm fertilize an egg. However, recent gene disruption experiments in mice have revealed that many factors previously described as important for fertilization are largely dispensable. One could argue that the fertilization mechanism is made robust against gene disruptions. However, this is not likely, as there are already six different gene-disrupted mouse lines （Calmegin, Adam Ia, Adam2, Adam3, Ace and Pgapl）, all of which result in male sterility. The sperm from these animals are known to have defective zona-binding ability and at the same time lose oviduct-migrating ability. Concerning spermzona binding, the widely accepted involvement of sugar moiety on zona pellucida 3 （ZP3） is indicated to be dispensable by gene disruption experiments. Thus, the landscape of the mechanism of fertilization is revolving considerably. In the sperm-egg fusion process, CD9 on egg and IZUMO1 on sperm have emerged as essential factors. This review focuses on the mechanism of fertilization elucidated by gene-manipulated animals.

Comparative transcriptome analysis of abalone Haliotis discus hannai with green and gray egg colors

Haliotis discus hannai is an important marine economic species in China.Its egg color was found to be associated with economic traits,which provides a new idea for breeding.However,the molecular mechanism of the egg-color formation has not been reported.Thus,the pigment composition and comparative transcriptome analyses of H.discus hannai with green and gray egg color were conducted using high-performance liquid chromatography(HPLC)and RNA-Seq methods.Results show that individuals with green and gray eggs both possess the fucoxanthin.Lutein existed in gray-egged individuals,but not in green-egged individuals.In transcriptome analysis,272310 unigenes were received from 461162 transcripts with a mean length of 985 bp and N50 of 1524 bp,respectively.A total of 185 unigenes were identifi ed as diff erentially expressed genes(DEGs).The DEGs involved in“fl avin-containing compound metabolic process”,“melanosome”,“glutathione metabolism”,and“cytochrome b6f complex”were likely related to the formation of the egg color.Our results provide foundational information for the functional analysis of egg-color related genes and are benefi cial to the selective breeding of H.discus hannai.

基于DNA条形码技术的珠江口春季鱼卵和仔稚鱼种类组成和分布特征的研究

采用线粒体COⅠ和12S rRNA基因片段作为DNA条形码,分析珠江口春季鱼卵和仔稚鱼种类组成和分布特征,并探究两种条形码在鱼卵和仔稚鱼种类鉴定中的适用性。研究共扩增样本391个,成功鉴定的鱼卵和仔稚鱼共7目25科42属60种(2种未鉴定到种)。其中,以鲈形目(Perciformes)种类和数量最多,种类数占比为51.6%,数量占比为47.91%;其次为鲱形目(Clupeiformes),种类数占比为25%,数量占比为34.56%。优势种10种,其中凤鲚(Coilia mystus)优势度最高,为0.071;棘头梅童鱼(Collichthys lucidus)最低,为0.014。COⅠ和12S rRNA基因片段扩增结果显示,鱼卵和仔稚鱼12S rRNA基因片段扩增成功率(95.60%)明显高于COⅠ基因(43.22%)。遗传距离和ABGD分析显示,COⅠ基因种内遗传距离为0~0.005(平均0.003),种间遗传距离为0.061~0.376(平均0.253),两者间存在明显的“条形码间隙”,ABGD划分结果与数据库比对结果一致;12S r RNA基因种内遗传距离为0~0.011(平均0.007),种间遗传距离为0.007~0.487(平均0.283),龟(Chelon haematocheila)和前鳞龟(Chelon affinis)种间遗传距离与种内遗传距离不形成“条形码间隙”,ABGD将其划分为同一种。系统发育分析显示,在种的分类阶元,所有物种均能聚为独立分支,得到有效区分。综上,线粒体COⅠ和12S rRNA条形码可有效鉴定珠江口大多数鱼卵和仔稚鱼,但是COⅠ基因扩增成功率较低,12S rRNA基因部分近缘物种存在区分困难的情况,两种基因结合使用更能提高鱼卵和仔稚鱼种类鉴定的成功率和准确性。

鸭蛋质量相关遗传变异及功能基因筛选与鉴定

本研究根据金定鸭个体蛋质量情况,选择2种极端表型,分为高蛋质量组(WH)和低蛋质量组(WL)。基于混池全基因组重测序和选择清除分析技术筛选组间差异显著基因组区域内的单核苷酸多态性(SNP)位点及相关功能基因,并通过单个样本重测序对筛选的蛋质量相关SNP进行验证,分析各SNP位点不同基因型之间的蛋质量大小差异。研究发现,在低蛋质量组和高蛋质量组获得的高质量reads数量分别为194115424和228089084,共定位到SNP差异显著区间178个,共富集到受选择候选基因40个,而且这些区间和基因均位于Z号染色体。鉴定出候选基因ARSB上Z-22908831、Z-22966695突变位点显著影响300 d、450 d蛋质量,RORB上Z-35251072、Z-35256947突变位点显著影响450 d蛋质量,RORB上Z-35278196突变位点显著影响300 d、450 d蛋质量,RASEF上Z-39588570突变位点显著影响450 d蛋质量。本研究结果为通过分子育种技术提高蛋鸭产蛋性能选育提供了依据,加快了选育进程。

不同饲育方式对家蚕产卵量及卵黄蛋白相关基因表达的影响

为探究人工饲料与桑叶不同搭配饲育方式对家蚕产卵情况及卵黄蛋白相关基因表达的影响,本研究采用全龄桑叶育(Mul1-5)、1~2龄人工饲料育+3~5龄桑叶育(Art1-2)、1~3龄人工饲料育+4~5龄桑叶育(Art1-3)、1~4龄人工饲料育+5龄桑叶育(Art1-4)4种饲育方式饲养菁松×皓月,调查不同饲育方式下的造卵量、产卵量、百粒卵重及卵黄蛋白基因Vg、30Kc19、ESP、VgR的表达情况。结果表明,Mul1-5的24 h产卵量、造卵量及百粒卵重均最高,造卵数量和百粒卵重都随人工饲料饲喂龄期延长呈现下降趋势;Mul1-5和Art1-2的造卵量显著高于Art1-3和Art1-4,Mul1-5的百粒卵重显著高于其他3个组合。利用荧光定量PCR方法测定了4种饲育方式下卵黄蛋白相关基因的表达情况,结果显示,Vg从5龄第7天开始到整个蛹期结束持续表达,整体表现为Art1-3的表达量最高,Art1-2的次之,Art1-4的最低;30Kc19在5龄第7天及上蔟第1天表达量较高,并分别以Art1-2和Art1-3方式下最高,蛹期基本不表达;ESP和VgR在整个蛹期都有表达,但以第5~8天的表达量较高,且第5~7天以Art1-4的最高,第8天以Art1-3的最高。综合来看,人工饲料育替代桑叶育的龄期越长,家蚕产卵数量和百粒卵重下降越明显,卵黄蛋白相关基因的表达受影响越大,这可能与人工饲料的配方、家蚕对人工饲料的吸收利用程度及人工饲料育后家蚕的体质有关,具体影响机制还需进一步研究。

鸽GnIH基因多态性及其与产蛋性状的关联分析

【目的】探究鸽促性腺激素抑制激素(gonadotropin-inhibitory hormone,GnIH)基因多态性,筛选影响母鸽产蛋性状的显著单核苷酸多态性(single nucleotide polymorphism,SNP)位点,用于高产母鸽的早期选择。【方法】本试验以78对白羽王鸽为研究对象,根据前期克隆获得的鸽GnIH基因mRNA序列(GenBank登录号:MG589639.1)设计引物,通过PCR扩增和直接测序法检测GnIH基因SNP位点并分型,使用Haploview软件对GnIH基因SNP进行连锁不平衡分析,使用SPSS 22.0软件对GnIH基因多态性与白羽王鸽产蛋性状进行关联分析。【结果】白羽王鸽GnIH基因中共检出7个SNPs,分别位于外显子1(c.59 C>T、c.72 T>A)、外显子2(c.398 G>C)和3′-UTR(c.768 C>T、c.860 G>A、c.909 A>G、c.961 T>C),除c.59 C>T位点偏离Hardy-Weinberg平衡外(P<0.05),其余位点均处于Hardy-Weinberg平衡状态(P>0.05);c.768 C>T与c.961 T>C位点呈完全连锁不平衡状态(D’=1,r 2=1),c.860 G>A与c.768 C>T、c.961 T>C位点呈强连锁状态(D’=1,r 2=0.69),其余位点呈弱连锁状态;c.398 G>C位点突变造成了氨基酸性质和mRNA二级结构的改变,该位点与母鸽年产蛋量和初产体重均呈显著相关(P<0.05)。【结论】GnIH基因外显子2上的SNP位点对母鸽产蛋性状有显著影响,可作为母鸽产蛋性能的候选分子标记。

捻转血矛线虫PCR检测方法的建立及其应用

为了能从粪便中对捻转血矛线虫卵进行特异性检测,基于捻转血矛线虫ITS2-28S基因序列设计特异性引物,通过对退火温度反应条件优化,建立捻转血矛线虫特异性PCR检测方法。结果显示,该方法成功从捻转血矛线虫卵中扩增出约270 bp的特异性片段,其最低检出质量浓度为0.298 pg/μL,敏感性较高;进一步对捻转血矛线虫、细颈线虫、粗纹食道口线虫等多种线虫的虫卵DNA样品进行扩增,该方法仅能特异性扩增出捻转血矛线虫卵的目的片段,证明特异性良好。利用所建立的PCR检测方法对120只山羊的粪便样品进行检测,显示受检样品中捻转血矛线虫阳性率为38.3%,高于显微镜检测结果(阳性率为24.2%)。结果表明,该研究建立的PCR方法能够应用于临床检测山羊粪便样品中的捻转血矛线虫卵,可为山羊捻转血矛线虫病的诊断与防治提供有效技术支持。