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51.
Homeobox (HOX) proteins are known for their critical role in body shape formation and tissue differentiation of developing vertebrate embryos. Recent research has shown that HOX proteins have many physiological roles such as cell proliferation, cell cycle, apoptosis and cell differentiation in adults, as well as the development of the vertebrate nerve and reproductive system. This study was conducted to determine the possible physiological functions and expression intensities of HOXA10, HOXA11, HOXB6 and HOXC6 proteins in the male reproductive system (testes, epididymis and deferens ducts), which are important for the continuity of some specific cat breeds in different age ranges. In the study, a total of 18 testicular tissues were used, divided into two groups: less than 6 months (immature) and more than 1 year (mature). Tissue samples were then subjected to immunohistochemical staining with protein-specific antibodies examined in the study. In the findings obtained in the research; it was observed that HOXA10, HOXA11, HOXB6 and HOXC6 produced different intensities of immunolocalization in the epididymis and ductus deferens layers in the immature and mature testicular cells. In addition, it was found that HOXA10 immunoreaction was also seen in some vascular endothelial cells. As a result, it was concluded that the HOX proteins could contribute to the physiological functions of testes, epididymis and ductus deferens and affect male fertility.  相似文献   
52.
旨在筛选出幼龄和成年太行山羊附睾头中差异表达的长链非编码RNAs(lncRNAs)、微小RNAs(miRNAs)和mRNAs,构建太行山羊附睾头中免疫相关基因调控的竞争性内源RNAs(ceRNAs)网络。本研究选取健康状况良好、体重相近的幼龄(2月龄)和成年太行山羊(2周岁)公羊各3只,去势采集其附睾头组织进行全转录组测序,用DESeq2软件筛选出幼龄和成年太行山羊附睾头差异mRNAs、lncRNAs和miRNAs。利用miRanda软件和R-package(reshape2、dplyr、tidyr),基于ceRNA-score原理分析得到差异ceRNAs表达谱,对预测所得具有ceRNAs关系的mRNAs进行GO和KEGG富集分析,并绘制得到太行山羊附睾头免疫相关ceRNAs网络。最后,各随机挑选8个mRNAs、miRNAs和lncRNAs,并通过qRT-PCR验证全转录组测序结果的准确性。根据分析结果,以幼龄太行山羊附睾头为对照,成年山羊附睾头差异表达mRNAs有6 461个,其中上调2 997个、下调3 464个;差异表达lncRNAs共有1 147个,其中703个上调、444个下调;差异表达miRNAs共有182个,其中81个上调、101个下调。共得到具有ceRNAs调控关系的lncRNAs 366个,其中上调213个,下调153个;mRNAs有3 131个,其中1 253个上调,1 878个下调;miRNAs有140个,其中48个上调,92个下调。分析具有ceRNAs机制的基因发现,表达量显著上调的与免疫相关的mRNAs:淋巴细胞抗原6复合位点蛋白G5B(LY6G5B)、脂质运载蛋白9(LCN9)、解整合素金属蛋白酶28(ADAM28)和粘蛋白15(MUC15)基因在成年太行山羊附睾头表达量高,且极显著高于幼龄太行山羊(P<0.01)。GO和KEGG富集分析表明,具有ceRNAs机制的差异表达基因富集在内质网蛋白加工通路、蛋白质输出通路、粘蛋白型O-聚糖生物合成通路、细胞外基质受体相互作用通路等。qRT-PCR验证结果表明,除chi-miR-320-3p外,其余差异表达的mRNAs、lncRNAs和miRNAs表达趋势与全转录组测序结果一致。附睾头免疫相关ceRNAs网络分析表明,lncRNA-MSTRG.22929.11、lncRNA-MSTRG.57822.5、lncRNA-MSTRG.26758.1、lncRNA-MSTRG.12113.3、lncRNA-MSTRG.59930.2等lncRNAs作为ceRNAs可以调控附睾头免疫相关基因表达。本研究筛选出了幼龄和成年太行山羊附睾头差异ceRNAs,挖掘并绘制了免疫相关的关键ceRNAs网络,这些lncRNAs作为ceRNAs可为太行山羊附睾头免疫调控机制研究提供参考依据。  相似文献   
53.
旨在研究免疫细胞在健康雄性牦牛附睾和输精管的分布。采用免疫组织化学和实时荧光定量(qRT-PCR)方法对幼龄(5~6月龄)及成年(3~4岁)牦牛附睾(头、体、尾)和输精管中CD68+巨噬细胞、CD3+ T淋巴细胞、CD79α+ B淋巴细胞、IgA+和IgG+浆细胞的分布特征及其表面标志分子的表达水平进行研究。结果显示:CD68+巨噬细胞、CD3+ T淋巴细胞、CD79α+ B淋巴细胞、IgA+和IgG+浆细胞主要分布在附睾管和输精管的上皮和间质;另外,CD68和CD3 mRNA和蛋白水平在各年龄组牦牛附睾头和附睾体显著高于附睾尾和输精管(P < 0.05),而CD79α、IgA和IgG mRNA和蛋白水平在附睾尾和输精管显著高于附睾头和附睾体(P < 0.05);此外,在成年牦牛附睾和输精管CD3、CD79α、IgA、IgG、CD68 mRNA和蛋白水平均显著高于幼龄牦牛(P < 0.05)。综上提示,牦牛附睾头可能主要是细胞免疫发生的位点,而附睾尾和输精管则主要进行体液免疫应答,此外,成年牦牛附睾和输精管的局部免疫可能更完善,以上数据为进一步研究高原牦牛局部生殖免疫和病理提供了形态学资料。  相似文献   
54.
Aquaporins (AQPs) are channel proteins that facilitate the transepithelial and bidirectional movement of water. AQP9 is an aquaporin that is expressed in the mammalian epididymis. This water transport contributes to epididymal sperm concentration. This study aimed to examine the morphology of epididymal epithelium in piglets and boars, as well as the expression and immunolocalization of AQP9. The piglets presented an epididymal epithelium in differentiation with principal, basal and apical cells. The cellular population of the epididymal epithelium in boars consisted of principal, basal, apical, clear and narrow cells. The migratory cells known as halo cells were observed in the epididymis of both piglets and boars. AQP9 expression presented differences between piglets and boars. Moderate intensity of AQP9 immunoreaction was observed in the apical border of the epididymal epithelium of the caput and cauda regions in the piglet epididymis. A moderate‐to‐intense reaction for AQP9 was observed in the nuclei of epithelial cells of the three epididymal regions in the boar epididymis. The region of the cauda epididymis showed reactivity for AQP9 also in the apical border of the epithelium. It is believed that the AQP9 is already functional in piglets at only 1 week of age and is more active, playing a pivotal role in the caput and cauda regions of the epididymis. Moreover, the intense AQP9 expression in the apical border of epithelial cells in the cauda region of the boar epididymis suggests a higher performance of AQP9 in this region, where sperm complete their maturation process, stored and concentrated.  相似文献   
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