FoxA2 and p53 regulate the transcription of HSD17B1 in ovarian granulosa cells of pigs     

Xiaolong Yuan  Xiaofeng Zhou  Xiwu Qiao  Qi Wu  Zhixiang Yao  Yao Jiang  Hao Zhang  Zhe Zhang  Xilong Wang  Jiaqi Li 《Reproduction in domestic animals》2021,56(1):74-82

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Three SNPs within exons of INHA and ACVR2B genes are significantly associated with litter size in Dazu black goats     

Shi-Zhi Wang  Guang-Xin E  Yan Zeng  Yan-Guo Han  Yong-Fu Huang  Ri-Su Na 《Reproduction in domestic animals》2021,56(6):936-941

The aim of this study was to analyse the association between single-nucleotide polymorphisms within INHA and ACVR2B and litter size in Dazu black goats. In total, twenty-two SNPs were genotyped in 190 individuals by SNaPshot and resequencing. The results showed that three SNPs (SNP_1, SNP_12 and SNP_13 in this study) were detected to have significant additive genetic effect on the recorded goat litter size (p < .05). The SNP_1 (NC_030809.1), a non-synonymous substitution of G for T at chr2-g. 28314990 in the exon 2 of INHA gene (NM_001285606.1), resulted in homozygote 2 (HOM2) contributed 0.25 and heterozygote (HET) contributed 0.12 larger litter than homozygote 1 (HOM1). Meanwhile, SNP_12 (Chr22-g. 11721225 A > T) and SNP_13 (Chr22-g. 11721227 A > C) (NC_030829.1) simultaneously mutated at the first and third position of a triplet AAA (lysine, K) in the exon 4 of ACVR2B gene (XM_018066623.1) had estimated genetic effects of HOM1 (0.00) and HOM2 (0.03) larger than HET (−0.12). In conclusion, one SNPs (chr2-g. 28314990 T > G) within the exon 2 of INHA and two SNPs (Chr22-g. 11721225 A > T and Chr22-g. 11721227 A > C) i n the exon 4 of ACVR2B gene were highly recommended as candidate markers of litter size in Dazu black goats. A large-scale association study to assess the impact of these variants on litter size is still necessary.  相似文献   

New Polyketides from the Antarctic Fungus Pseudogymnoascus sp. HSX2#-11     

Ting Shi  Yan-Yan Yu  Jia-Jia Dai  Yi-Ting Zhang  Wen-Peng Hu  Li Zheng  Da-Yong Shi 《Marine drugs》2021,19(3)

The species Pseudogymnoascus is known as a psychrophilic pathogenic fungus with a ubiquitous distribution in Antarctica. Meanwhile, the study of its secondary metabolites is infrequent. Systematic research of the metabolites of the fungus Pseudogymnoascus sp. HSX2#-11, guided by the method of molecular networking, led to the isolation of one novel polyketide, pseudophenone A (1), along with six known analogs (2–7). The structure of the new compound was elucidated by extensive spectroscopic investigation and single-crystal X-ray diffraction. Pseudophenone A (1) is a dimer of diphenyl ketone and diphenyl ether, and there is only one analog of 1 to the best of our knowledge. Compounds 1 and 2 exhibited antibacterial activities against a panel of strains. This is the first time to use molecular networking to study the metabolic profiles of Antarctica fungi.  相似文献   

Identification of an H1N1 subtype of swine influenza virus and serological analysis     

Fa-chao SUN  Min TAN  Yuan-chao ZHANG  Yu-chao WANG  Sheng-liang CAO  Guo-fei DING  Fang-yuan CONG  Li-hong GUO  Si-dang LIU  Yi-hong XIAO 《农业科学学报》2019,18(7):1436-1442

To investigate the epizootic of swine influenza virus(SIV), 60 nasal swabs were collected from a clinical cases of pig farm in Tai'an City, Shandong Province of China in April 2017. SIV was isolated by inoculating into 10-day-old Special Pathogen Free embryonated eggs and the whole genome was sequenced. An H1N1 subtype SIV was isolated and designated as A/swine/Shandong/TA04/2017(H1N1). Phylogenetic analysis showed that apart from the polymerase A(PA) fragment belonging to the 2009 pandemic H1N1 branch, seven genome segments belonged to avian-like H1N1 influenza virus lineage. The cleavage site sequence of the hemagglutinin(HA) protein was PSIQSR↓G, which is a typical molecular biological characteristic. Five potential N-glycosylation sites(N14, N26, N277, N484 and N543) were found in the HA gene. To further investigate the epidemiology of SIV in this farm, the 995 serum samples were assessed with EAH1N1 2009 pandemic H1N1 and H3 N2 antigens. The results showed that the total positive rate was 65.43%. The positive rates of single virus infection detected by EAH1N1, 2009 pdmH1N1 and H3 N2 for serum HI(Hemagglutination inhibition) were 48.35, 30.85 and 7.47%, respectively. The results showed that SIV in Shandong Province has been reassorted in some segments and the SIV-positive rate was high on the SIV outbreak farm. These data provide evidence of an epizootic of SIV.  相似文献   

预防兽医学分子生物学技术发展概况   总被引：6，自引：2，他引：4  

景志忠  才学鹏  陈娟 《动物医学进展》2002,23(4):10-14

概括介绍了分子生物学理论、技术的发展，重点从病原学、免疫学和疫病预防与控制学三方面阐述了分子生物学在预防兽医学中的应用、发展及其贡献。同时，阐明了预防兽医学对分子生物学的贡献和促进作用。  相似文献   

分子间的作用及其结构适应性   总被引：3，自引：0，他引：3  

郭世豪 《湖南农业大学学报(自然科学版)》2001,27(2):148-150

某些分子间的作用无法的用范德华力、氢键、介电常数、偶极矩等化学基本理论来加以解释，引入控制论的方法对这些分析间的作用进行研究后的结果表明，选择性分析间引力很可能是分子是最强的物理作用，而分子间的化学作用亦与分子间的结构适应性密切相关。  相似文献   

分子标记用于赤眼蜂分子监测的研究   总被引：5，自引：0，他引：5  

李正西  沈佐锐 《农业生物技术学报》2001,9(1):65-68

通过对松毛虫赤眼蜂（Trichogramma dedrolimi Matsumura）以及玉米螟赤眼蜂（Trichogramma ostriniae Pang et Chen）rDNA-ITS2基因的克隆测序，并联机检索GenBank核酸序列库中其它赤眼蜂的相关序列，利用核酸分析软件找到松毛虫赤眼蜂和玉米螟赤眼蜂ITS2序列中一段有鉴别意义的标志，并据此设计出蜂种的特异PCR引物，实现了松毛虫赤眼蜂和玉米螟赤眼蜂rDNA特异区带的PCR扩增。研究表明该特异区带具有种的特异性。我们认为该分子标记技术可用于目前我国生防中常用的松毛虫赤眼蜂和玉米螟蒌眼蜂的分子监测，如田间种群动态监控和寄生效果评估。  相似文献   

用RAPD技术筛选中国荷斯坦牛产奶量性状遗传标记   总被引：10，自引：3，他引：7  

杜立新  万海伟  王爱华  李宏滨 《畜牧兽医学报》2005,36(9):882-886

选用320条10碱基随机引物在由36头高产（305d产奶量〉8500kg）和32头低产（305d产奶量〈5600kg）中国荷斯坦牛所组成的2个DNA池间进行RAPD-PCR扩增，从中筛选出稳定性好、带型清晰且在2个DNA池间有明显差异的RAPD引物24条。用筛选到的24条引物对所有个体进行PCR检测，得到了5个与奶牛产奶量性状相关的RAPD标记，并对其中4个进行了克隆测序和SCAR标记转化以及生物信息学分析。结果表明：SCAR标记yield—s139与产奶量密切相关，应用电子克隆方法已将该标记由921bp延伸到2141bp，经同源性比较发现，此标记对应于奶牛基因组中LINEs家族中的一个重复元件，推测该元件附近可能存在与产奶量性状相关的QTLs或主效基因。  相似文献   

牛Myostatin基因单核苷酸多态性分析     

史明艳  昝林森  李保兰  刘霞  张自富 《勤云标准版测试》2005,(6)

Myostatin基因即肌肉生长抑制素,是一种肌肉生长的负调控因子。应运PCR-SSCP和测序的方法对中国秦川牛、南阳牛以及国外引入品种皮埃蒙特牛双肌基因的第三外显子进行了多态性分析。结果表明:第三外显子938处G→A的单核苷酸的突变造成了南阳牛、皮埃蒙特牛第三外显子扩增片段多态性,秦川牛则不然。  相似文献   

RT-PCR及RFLP分析技术对鸡传染性支气管炎病毒的诊断和S1基因分型的研究   总被引：4，自引：0，他引：4  

磨美兰  李康然  韦平 《中国预防兽医学报》2001,23(4)

本研究使用分别扩增整个S1糖蛋白基因 (引物A)和S1糖蛋白基因N_端高变区Ⅰ (引物B)的 2对引物对 3个IBV标准株M41、Connecticut、Arkansas及 5个地方分离株 (C60 ,D41A ,D41B ,A112 1,A1171)进行RT_PCR扩增。用引物A时 ,有 5个IBV毒株扩增到目的片段 (172 0bp) ;用引物B时 ,所有 8个IBV毒株均得到与预计大小相符的目的产物 (2 2 8bp)。对 172 0bp的PCR产物用限制性内切酶HaeⅢ进行酶切 ,结果得出 3个不同的RFLP图谱 ,其中M41、Connecticut、D41B具有相同的HaeⅢ酶切图谱。Arkansas和D41A则分别具有互不相同的图谱 ;对 2 2 8bp的PCR产物进行DdeⅠ、RsaⅠ限制性内切酶消化 ,根据它们的RFLP图谱 ,8个IBV毒株可分为 5个基因型。综合 2对引物的PCR产物的RFLP分析结果 ,8个IBV毒株可分为 7个基因型 ,分型的结果与传统的血清学方法吻合。本研究建立的方法和技术具有快速、简单、特异、灵敏等优点 ,为现场流行毒株的定型(基因型 /血清型 )及其S1基因变异的跟踪研究以及更有效防制传染性支气管炎奠定了基础。  相似文献