miR-23b-3p通过靶向PDE4B基因调控山羊肌内前体脂肪细胞的分化

本研究旨在明确miR-23b-3p对山羊肌内前体脂肪细胞分化的影响，并确定这种作用是通过靶向基因PDE4B来实现的。基于实验室前期转录组测序结果，以筛选得到的山羊肌内脂肪细胞分化前后差异表达的miR-23b-3p为切入点，利用实时荧光定量PCR (real-time quantitative-polymerase chain reaction, qPCR)技术检测miR-23b-3p在山羊肌内前体脂肪细胞分化过程中的表达模式，从形态学水平和分子水平确定miR-23b-3p对脂肪分化及脂肪分化标志基因的影响；利用生物信息学预测以及双荧光素酶报告基因试验确定miR-23b-3p的下游靶基因，明确miR-23b-3p与预测靶标基因的靶向关系。结果表明，过表达miR-23b-3p后山羊肌内脂肪细胞脂滴积聚减少，成脂标志基因AP2、C/EBPα、FASN、LPL表达水平极显著下调(P＜0.01)，C/EBPβ、DGAT2、GLUT4和PPARγ的表达水平显著下调(P＜0.05)。干扰miR-23b-3p表达后，山羊肌内脂肪细胞中脂滴积聚增多，ACC、ATGL、AP2、DGAT2、GLUT4、FASN和SREBP1表达水平极显著上调(P＜0.01)，C/EBPβ、LPL和PPARγ的表达水平显著上调(P＜0.05)。通过生物信息学分析预测，PDE4B可能为miR-23b-3p的靶标基因，且过表达miR-23b-3p后极显著降低PDE4B的mRNA表达水平(P＜0.01)，干扰miR-23b-3p后PDE4B的mRNA水平得到了显著提升(P＜0.05)。双荧光素酶报告基因试验结果表明，miR-23b-3p与PDE4B基因存在靶向关系。miR-23b-3p通过靶向PDE4B基因调控山羊肌内前体脂肪细胞的分化。     

鸡zp1基因对成骨细胞矿化的影响

本研究旨在克隆编码鸡透明带1（zona pellucida 1,Zp1）蛋白的zp1基因,并研究其组织表达谱及在成骨细胞矿化中的作用。利用实时荧光定量聚合酶链式反应（real-time fluorescence quantitative polymerase chain reaction,RT-qPCR）检测蛋鸡不同组织和性成熟启动前后胫骨中的zp1表达水平;将Zp1过表达载体转染至诱导分化8 d的鸡颅骨成骨细胞内,检测细胞外矿化基质和矿化相关基因表达。结果表明,鸡zp1基因全长3 045 bp,编码958个氨基酸残基,具有2个N-糖基化位点。zp1基因在产蛋期鸡肝脏中高水平表达,其次为胫骨和卵黄膜,在蛋壳腺和心脏中不表达。鸡性成熟启动后血浆雌激素（estrogen,E2）、胫骨糖胺聚糖（glycosaminoglycan,GAG）含量和zp1表达量均极显著高于性成熟启动前。在过表达Zp1的鸡成骨细胞中添加雌激素后,细胞外矿化基质和矿化相关基因表达水平均显著升高。因此,zp1基因表达具有组织特异性,在雌激素作用下正向调控鸡成骨细胞矿化,为阐明Zp1在鸡产蛋期骨骼中的功能特性奠定了理论基础。     

核桃JrsHSP17.3基因克隆及温度胁迫响应模式分析

通过分析核桃（Juglans regia）转录组,鉴定获得核桃热激蛋白家族sHSP17.3基因的全长cDNA序列,命名为JrsHSP17.3。JrsHSP17.3基因开放读码框474 bp,编码产物含157个氨基酸,分子量为17.64 kD,理论等电点为5.35。为了研究该基因表达的组织特异性及温度响应模式,采用实时荧光定量PCR（qRT-PCR）方法,对高温和低温胁迫下JrsHSP17.3基因在根、茎、叶中的转录水平进行分析。结果显示,JrsHSP17.3基因在不同组织中均有表达;经高温（36 ℃～52 ℃）和低温（16 ℃～6 ℃）处理后,JrsHSP17.3基因均可被显著诱导,其中12 ℃胁迫1 h表达最高,为对照（非处理情况）的142.02倍。研究表明核桃JrsHSP17.3基因能够响应冷热温度胁迫,为进一步研究JrsHSP17.3基因的抗寒耐高温特性奠定基础。     

不同代次牛成肌细胞的诱导分化及相关基因的表达分析

利用初生荷斯坦牛的成肌细胞,在不同代次以含体积分数为2%马血清的DMEM进行诱导分化,在之后0、2、4、6、8、10 d观察细胞的形态变化并收集细胞提取总RNA,检测成肌相关基因的表达情况,为进一步研究牛肌肉发生过程及相关基因的表达调控提供依据。同时利用实时荧光定量PCR分别检测肌性相关基因MyoD(生肌决定因子)、MyoG(肌细胞生成素)以及非肌性相关基因A-FABP(脂肪细胞型脂肪酸结合蛋白)表达水平的变化。研究表明：①各代细胞在诱导培养4 d后开始有肌管形成,其后越来越多,8 d时达高峰。②成肌细胞向成熟肌细胞分化过程中,MyoD、MyoG、A-FABP基因都呈先上升然后下降的趋势。③高代次成肌细胞比低代次细胞增殖慢,而且在诱导分化后,肌管的数目明显变少; MyoD、MyoG、A-FABP随着代次的升高而下降。故推断MyoD、MyoG以及A-FABP基因会在成肌分化开始后的不同阶段被激活,从而发挥不同的调控作用,而且随着传代次数的增加成肌细胞的分化能力减弱。     

基于CRISPR/Cas9系统构建绵羊VASA基因敲入载体及验证

本研究旨在探索VASA基因在绵羊睾丸发育中的表达变化,并通过构建VASA基因敲入载体,为下一步进行绵羊生殖细胞体外诱导分化研究提供基础。采集性成熟前后即3月龄（3-month-old,3M）和9月龄（9-month-old,9M）绵羊睾丸组织,利用实时荧光定量PCR （quantitative real-time PCR,qPCR）和Western blotting技术分析VASA基因的差异表达,并利用免疫组织化学技术对VASA基因的表达定位进行分析。设计靶向VASA基因的向导RNA （guide RNA,gRNA）,并构建同源重组载体,进行质粒转染绵羊耳成纤维细胞。结合CRISPR/dCas9技术对VASA基因进行激活,进一步验证载体效率。结果表明,VASA基因随着绵羊睾丸发育,表达水平极显著增加（P<0.01）,且主要定位在精母细胞和圆形精子细胞中。利用CRISPR/Cas9系统构建了VASA基因敲入载体,联合pEGFP-PGK puro-VASA载体转染耳成纤维细胞,CRISPR/dCas9系统激活后,耳成纤维细胞成功表达VASA基因。结果提示,VASA基因在绵羊睾丸发育和精子发生中发挥潜在功能,且通过CRISPR/Cas9系统可在体外构建VASA基因敲入载体,为下一步探究VASA基因对绵羊雄性生殖细胞的发育和分化提供有效的研究手段。     

矮牵牛PhTPS5基因的克隆与表达分析

海藻糖 6 磷酸合成酶（Trehalose 6 phosphate synthase）基因TPS是海藻糖生物合成途径中的关键基因之一。该研究从矮牵牛 (Petunia hybrida)中分离了TPS5的同源基因PhTPS5。该基因开放阅读框（ORF）为2 595 bp,编码864个氨基酸。推测PhTPS5蛋白的分子式为C⁴³⁶³H⁶⁸²⁵N¹¹⁷³O¹²⁸⁹S³⁷。组织特异性表达分析显示：PhTPS5基因在根中表达量最高,叶片中的表达量最低;去顶6 h能够显著促进PhTPS5基因的表达,但24 h后表达量明显下降;去顶后施加生长素则能够有效抑制去顶对PhTPS5基因表达的调节;施加细胞分裂素6 h后PhTPS5基因的表达水平显著上调,但随着处理时间的增加,其表达水平有所下降。该研究为进一步揭示TPS途径在矮牵牛分枝发育中的调控机制奠定了理论基础。     

利用Red系统快速敲除家蚕核型多角体病毒orf60基因

用Red重组系统和最近构建的家蚕核型多角体病毒（BmNPV）bacmid在大肠杆菌BW25113中快速地敲除BmNPV orf60基因。从大肠杆菌BmDH10Bac中提取BmNPV bacmid,将其电转化到含有质粒pKD46（能表达Red重组酶）的大肠杆菌菌株BW25113中,获得了可用于BmNPV基因打靶的菌株BW25113-Bac。设计一对长63bp的引物（5′端为orf60基因的左右同源臂,长45bp;3′端长18bp,为氯霉素抗性基因（cat）的首尾序列）,以pKD3质粒（含cat）为模板,PCR扩增携带orf60左右同源臂的cat,即打靶线性化片段。将该线性化片段电转入BW25113-Bac菌株,在Red重组酶的作用下,线性化片段与BmNPV bacmid中的orf60基因发生同源重组。设计3对特异引物,用PCR方法证明cat成功地替换了BmNPV orf60基因。重组bacmid DNA转染BmN细胞后,Western blot分析未检测到orf60基因的表达。     

鼠mPC-1基因的克隆与特性分析

为深入研究人前列腺癌相关基因PC-1的生物功能和进化保守状况,从小鼠肾脏中克隆了全长cDNA序列,命名为mPC-1（GenBank Acc No.AY048852）.mPC-1基因cDNA全长为2 193 bp,主要定位于小鼠染色体3A1-A2区域.mPC-1基因最大开放阅读框编码的蛋白质由224个氨基酸组成,与人PC-1蛋白编码区存在82%的序列一致性,含有coiled-coil结构域和PEST结构域.生物信息学分析表明,由6个外显子组成的mPC-1基因与mD52高度同源,其中,第一外显子代表该基因的特异性序列,实验证据显示mPC-1基因具有自己的启动子,推测mPC-1与小鼠mD52可能是重叠基因.对小鼠20种组织器官和不同发育阶段的胚胎组织cDNA的RT-PCR检测证实,该基因主要在前列腺、肾和眼组织中表达,在胃和平滑肌中有少量表达,在其他组织中表达很弱或不表达.而mD52基因则几乎广泛存在于小鼠的各个组织器官中,因此,两个基因虽然序列上高度重叠却是独立调控的.综上所述,mPC-1基因可能是一个与人PC-1基因结构功能类似的新基因.     

Adipose triglyceride lipase regulates lipid metabolism in dairy goat mammary epithelial cells

Adipose triglyceride lipase (ATGL) catalyzes the initial step in the lipid lipolysis process, hydrolyzing triglyceride (TG) to produce diacylglycerol (DG) and free fatty acids (FFA). In addition, ATGL regulates lipid storage and release in adipocyte cells. However, its role in mammary gland tissue remains unclear. To assess the role of the ATGL gene in the goat mammary gland, this study analyzed the tissue distribution and expression of key genes together with lipid accumulation after knockdown of the ATGL gene. The mRNA of ATGL was highly expressed in subcutaneous adipose tissue, the lung and the mammary gland with a significant increase in expression during the lactation period compared with the dry period of the mammary gland. Knockdown of the ATGL gene in goat mammary epithelial cells (GMECs) using siRNA resulted in a significant decrease in both ATGL mRNA and protein levels. Silencing of the ATGL gene markedly increased lipid droplet accumulation and intracellular TG concentration (P < 0.05), while it reduced FFA levels in GMECs (P < 0.05). Additionally, the expression of HSL for lipolysis, FABP3 for fatty acid transport, PPARα for fatty acid oxidation, ADFP, BTN1A1, and XDH for milk fat formation and secretion was down-regulated (P < 0.05) after knockdown of the ATGL gene, with increased expression of CD36 for fatty acid uptake (P < 0.05). In conclusion, these data suggest that the ATGL gene plays an important role in triglyceride lipolysis in GMECs and provides the first experimental evidence that ATGL may be involved in lipid metabolism during lactation.     

Polymorphisms of caprine <Emphasis Type="Italic">GDF</Emphasis>9 gene and their association with litter size in Jining Grey goats

The exons 1, 2 and flanking region of growth differentiation factor 9 (GDF9) gene in five randomly selected does of Jining Grey, Boer and Liaoning Cashmere goats were amplified and analyzed. Thirteen nucleotide differences were identified in GDF9 gene between sheep (AF078545) and goats. Four SNPs (G3288A in intron 1, G423A, A959C [Gln320Pro] and G1189A [Val397Ile] in exon 2) were detected in four goat breeds with different prolificacy, in which G3288A was a new SNP in goats. The results showed that loci 3288, 423 and 1189 in Boer goats, loci 3288 and 423 in Guizhou White goats, loci 423 and 1189 in Liaoning Cashmere goats were all in complete linkage disequilibrium (D′ = 1, r ² = 1), respectively. In moderate (Boer goat) and low prolificacy (Liaoning Cashmere goat) breeds, linkage analysis indicated that there were more fervent linkage disequilibrium among loci 3288, 423 and 1189 than high prolificacy (Jining Grey and Guizhou White goats) breeds. For the 959 locus, the genotype distribution showed obvious difference between high prolificacy breeds and moderate or low prolificacy breeds (P < 0.05 or P < 0.01). The Jining Grey goat does with genotype CC or AC had 0.81 (P < 0.01) or 0.63 (P < 0.01) kids more than those with genotype AA, respectively. The present study preliminarily showed an association between allele C at 959 locus of GDF9 gene and high litter size in Jining Grey goats. These results provide further evidence that the GDF9 gene may be significantly correlated with high prolificacy in goats.     

Identification and characterization of adipose triglyceride lipase (ATGL) gene in birds

Adipose triglyceride lipase (ATGL) is a triglyceride hydrolysis lipase and is generally related to lipid metabolism in animals. The ATGL gene was well studied in mammals, however very less was known in birds that differed significantly with mammals for lipid metabolism. In this study, cloning, mRNA real time and association analysis was performed to characterize the ATGL gene in birds. Results showed that the obtained ATGL gene cDNA of parrot, quail, duck were 1,651 bp (NCBI accession number: GQ221784), 1,557 bp (NCBI accession number: GQ221783) and 1,440 bp each, encoded 481-, 482- and 279-amino acid (AA) peptide, respectively. The parrot ATGL (pATGL) gene was found to predominantly express in breast muscle and leg muscle, and very higher ATGL mRNA level was also found in heart, abdominal fat and subcutaneous fat. The quail ATGL (qATGL) gene was also predominantly expressed in breast muscle and leg muscle, and then to a much lesser degree in heart. The duck ATGL (dATGL) gene was found to predominantly express in subcutaneous fat and abdominal fat, quite higher ATGL mRNA was also found in heart, spleen, breast muscle and leg muscle. Blast analyses indicated the high homology of ATGL and its patatin region, and moreover, and the active serine hydrolase motif (“GASAG” for “GXSXG”) and the glycine rich motif (“GCGFLG” for “GXGXXG”) were completely conservative among 14 species. Association analyses showed that c.950+24C>A, c.950+45C>G, c.950+73G>A, c.950+83C>T and c.950+128delA of chicken ATGL gene (cATGL) were all significantly or highly significantly with cingulated fat width (CFW) (P < 0.05 or P < 0.01), and c.777−26C>A, c.950+45C>G, c.950+73G>A and c.950+118C>T were all significantly or highly significantly with pH value of breast muscle (BMPH) (P < 0.05).     

Molecular characterization of fibroblast growth factor-16 and its role in promoting the differentiation of intramuscular preadipocytes in goat

Fat metabolism is an important and complex biochemical reaction in vivo and is regulated by many factors. Recently, the findings on high expression of fibroblast growth factor-16 (FGF16) in brown adipose tissue have led to an interest in exploring its role in lipogenesis and lipid metabolism. The study cloned the goat’s FGF16 gene 624 bp long, including the complete open reading frame that encodes 207 amino acids. We found that FGF16 expression is highest in goat kidneys and hearts, followed by subcutaneous fat and triceps. Moreover, the expression of FGF16 reached its peak on the 2nd day of adipocyte differentiation (P < 0.01) and then decreased significantly. We used overexpression and interference to study the function of FGF16 gene in goat intramuscular preadipocytes. Silencing of FGF16 decreased adipocytes lipid droplet aggregation and triglyceride synthesis. This is in contrast to the situation where FGF16 is overexpressed. Furthermore, knockdown of FGF16 also caused down-regulated expression of genes associated with adipocyte differentiation including CCAAT enhancer-binding protein beta (P < 0.01), fatty acid-binding protein-2 (P < 0.01) and sterol regulatory element binding protein-1 (P < 0.05), but the preadipocyte factor-1 was up-regulated. At the same time, the genes adipose triglyceride lipase (P < 0.01) and hormone-sensitive lipase (P < 0.05) associated with triglyceride breakdown were highly expressed. Next, we locked the fibroblast growth factor receptor-4 (FGFR4) through the protein interaction network and interfering with FGF16 to significantly reduce FGFR4 expression. It was found that the expression profile of FGFR4 in adipocyte differentiation was highly similar to that of FGF16. Overexpression and interference methods confirmed that FGFR4 and FGF16 have the same promoting function in adipocyte differentiation. Finally, using co-transfection technology, pc-FGF16 and siRNA-FGFR4, siRNA2-FGF16 and siRNA-FGFR4 were combined to treat adipocytes separately. It was found that in the case of overexpression of FGF16, cell lipid secretion and triglyceride synthesis showed a trend of first increase and then decrease with increasing interference concentration. In the case of interference with FGF16, lipid secretion and triglyceride synthesis showed a downward trend with the increase of interference concentration. These findings illustrated that FGF16 mediates adipocyte differentiation via receptor FGFR4 expression and contributed to further study of the functional role of FGF16 in goat fat formation.     

Knockdown of KLF9 promotes the differentiation of both intramuscular and subcutaneous preadipocytes in goat

ABSTRACT

KLF9 is reported to promote adipocyte differentiation in 3T3-L1 cells and pigs. However, the roles of KLF9 in adipocytes differentiation of goat remain unknown. In this study, the expression profiles of KLF9 were different between subcutaneous and intramuscular preadipocytes of goat during differentiation process. After silencing KLF9 gene, the lipid droplets were increased in both two types of adipocytes. In subcutaneous preadipocyte with silencing KLF9, the expressions of C/EBPβ, PPARγ, LPL, KLF1-2, KLF5, and KLF17 genes were up-regulated, while KLF12, KLF4, and KLF13 genes were down-regulated in expression level. In intramuscular preadipocyte, aP2, C/EBPα, KLF2-3, KLF5, and KLF7 gene were up-regulated, and Pref-1 gene was down-regulated. In addition, the binding sites of KLF9 existed in the promoters of aP2, C/EBPα, C/EBPβ, LPL and Pref-1. Taken together, KLF9 play a negative role in the differentiation of both intramuscular and subcutaneous preadipocytes in goats, but the functional mechanism may be different.     

Polymorphisms of caprine <Emphasis Type="Italic">POU1F1</Emphasis> gene and their association with litter size in Jining Grey goats

Seven pairs of primers were designed to amplify 5′ promoter region, six exons and partial introns and to detect the polymorphisms of POU1F1 gene in five goat breeds with different prolificacy. The results showed that six mutations were identified in caprine POU1F1 gene including C256T in exon 3, C53T and T123G in intron 3, and G682T (A228S), T723G and C837T in exon 6. The former four mutations were novel SNPs in goat POU1F1 gene. The 53 and 123 loci were in complete linkage disequilibrium in five caprine breeds. Regarding the 256 locus, the Jining Grey goat does with genotype CT had 0.66 kids more than those with genotype CC (P < 0.05), while does with genotype GT had 0.63 (P < 0.05) kids more than those with genotype GG at the 682 locus. The present study preliminarily showed an association between allele T at the 256 and 682 loci of POU1F1 gene and high litter size in Jining Grey goats. Totally 16 haplotypes and 50 genotypes were identified at the above six loci in POU1F1 gene of five goat breeds. Three common haplotypes (hap2, hap3 and hap4) were identified in five goat breeds joined. Four specific haplotypes (hap7, hap9, hap11 and hap13) were detected in Jining Grey goats. The predominant haplotype was hap1 (35.29% and 48.25%) in both Jining Grey and Guizhou White goats, while hap4 (50%) in Boer goats, and hap2 (42.86% and 38.75%) in both Wendeng Dairy and Liaoning Cashmere goats. The most frequent genotypes at six loci in the above five goat breeds were hap1/hap2 (14.38%) and hap1/hap4 (14.38%), hap1/hap2 (38.60%), hap4/hap4 (40.91%), hap2/hap4 (26.53%), hap2/hap5 (20.00%), respectively. The Jining Grey goat does with nine genotypes analyzed of POU1F1 gene showed no obvious difference in litter size.     

lncRNA-H19/miR-29a axis affected the viability and apoptosis of keloid fibroblasts through acting upon COL1A1 signaling

This study was intended to clarify the potential of applying the long-chain noncoding RNA H19/miR-29a axis in keloid treatment by elucidating its correlation with the activity of fibroblasts. In this study, 80 keloid tissues, 63 normal fibrous tissues, and 91 normal skin tissues were collected in advance, and concurrently, fibroblasts separated from the tissues were cultured. Besides this, the si-H19, pcDNA3.1-H19, miR-29a mimic, and miR-29a inhibitor were transfected to keloid fibroblasts, whose proliferation, apoptosis, and metastasis were appraised by employing the colony formation assay, flow cytometry, and transwell assay. In addition, the luciferase reporter gene assay was carried out to determine whether targeted regulation was present between H19 and miR-29a, as well as between miR-29a and COL1A1. The study results demonstrated that keloid tissues and fibroblasts exhibited observably upregulated H19 expression and downregulated miR-29a expression, relative to normal skin tissues and fibroblasts (P < .05). Also observed was a negative correlation between H19 expression and miR-29a expression among the gathered keloid tissues (r_s = −.267, P = .017). Furthermore, in vitro transfection of pcDNA3.1-H19 or miR-29a inhibitor could intensify viability, proliferation, migration, and invasion of the fibroblasts (P < .05), while silencing of H19 and overexpression of miR-29a hindered both metastasis and multiplication of the fibroblasts significantly (P < .05). In addition, H19 was capable of altering miR-29a expression within fibroblasts by directly sponging it, and overexpression of COL1A1 could deter the impact of miR-29a on viability, proliferation, migration, and invasion of fibroblasts (P < .05). In conclusion, H19 might facilitate proliferation and metastasis of fibroblasts by modifying downstream miR-29a and COL1A1, which was expected to allow for development of keloid-targeted treatments.     

Analysis on DNA sequence of <Emphasis Type="Italic">GPR54</Emphasis> gene and its association with litter size in goats

The kisspeptin/GPR54 pathway is crucial in the process of puberty onset. Six pairs of primers were designed to clone goat GPR54 and scan polymorphisms and one pair of primers to detect polymorphisms of GPR54 in sexual precocious and sexual late-maturing goat breeds. A DNA fragment of 4258 bp of goat GPR54 was obtained, which contains an open reading frame (ORF) of 1137 bp and encodes 378 amino acids, having a high homology with other mammals. The protein was predicted to have seven transmembrane regions. There were no base pair variation in exons 1–4 and three base changes (G4014A, G4136A and C4152T) in exon 5 by sequencing and the three mutations may have some correlation with sexual precocity in goats. For the 4152 locus, the Jining Grey goat does with genotype TT and CT had 1.02 and 0.84 (P < 0.01) kids more than those with genotype CC, respectively. No significant difference (P > 0.05) was found in litter size between TT and CT genotypes in Jining Grey goat. For the other two loci, no significant difference (P > 0.05) was found in litter size between different genotypes in Jining Grey goats. The present study preliminarily indicated an association between allele T of the 4152 locus in GPR54 and high litter size in Jining Grey goats.