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An efficient and rapid method to detect and verify natural antisense transcripts of animal genes
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作者 ZHANG Li ZHAO Rui +8 位作者 XIAO Mei LIN Shu-dai LI Bi-xiao QIU Feng-fang ma jing-e ZHANG De-xiang NIE Qing-hua AN Li-long ZHANG Xi-quan 《Journal of Integrative Agriculture》 SCIE CAS CSCD 2016年第9期2070-2076,共7页
High-throughput sequencing has identified a large number of sense-antisense transcriptional pairs, which indicates that these genes were transcribed from both directions. Recent reports have demonstrated that many ant... High-throughput sequencing has identified a large number of sense-antisense transcriptional pairs, which indicates that these genes were transcribed from both directions. Recent reports have demonstrated that many antisense RNAs, especially lnc RNA(long non-coding RNA), can interact with the sense RNA by forming an RNA duplex. Many methods, such as RNA-sequencing, Northern blotting, RNase protection assays and strand-specific PCR, can be used to detect the antisense transcript and gene transcriptional orientation. However, the applications of these methods have been constrained, to some extent, because of the high cost, difficult operation or inaccuracy, especially regarding the analysis of substantial amounts of data. Thus, we developed an easy method to detect and validate these complicated RNAs. We primarily took advantage of the strand specificity of RT-PCR and the single-strand specificity of S1 endonuclease to analyze sense and antisense transcripts. Four known genes, including mouse β-actin and Tsix(Xist antisense RNA), chicken LXN(latexin) and GFM1(Gelongation factor, mitochondrial 1), were used to establish the method. These four genes were well studied and transcribed from positive strand, negative strand or both strands of DNA, respectively, which represented all possible cases. The results indicated that the method can easily distinguish sense, antisense and sense-antisense transcriptional pairs. In addition, it can be used to verify the results of high-throughput sequencing, as well as to analyze the regulatory mechanisms between RNAs. This method can improve the accuracy of detection and can be mainly used in analyzing single gene and was low cost. 展开更多
关键词 natural antisense transcripts transcription orientation detection method RNA sequencing long non-coding RNA
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茶多酚缓解脂多糖诱导肉鸡肠道炎症的微生态机制研究
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作者 李金 马荆鄂 王樟凤 《江西农业学报》 2025年第10期98-103,共6页
研究了茶多酚对脂多糖诱导肉鸡肠道炎症应激后的缓解作用,选择1日龄白羽肉鸡240只,随机分为4组:对照组(CK)、脂多糖(LPS)组、茶多酚(TP)组、茶多酚(TP)+脂多糖(LPS)组,其中TP组和TP+LPS组饲喂基础日粮并添加350 mg/kg茶多酚;试验第21天,... 研究了茶多酚对脂多糖诱导肉鸡肠道炎症应激后的缓解作用,选择1日龄白羽肉鸡240只,随机分为4组:对照组(CK)、脂多糖(LPS)组、茶多酚(TP)组、茶多酚(TP)+脂多糖(LPS)组,其中TP组和TP+LPS组饲喂基础日粮并添加350 mg/kg茶多酚;试验第21天,将LPS组、TP+LPS组腹腔注射脂多糖,试验期为26d。结果显示:LPS刺激了模拟肉鸡肠道炎症,促炎细胞因子和肿瘤坏死因子-α含量得到了显著提高,但添加TP对此具有恢复作用。添加TP和LPS刺激对肉鸡血清单核细胞趋化蛋白-1存在显著的交互作用。LPS刺激显著降低了肉鸡盲肠厚壁菌门、提高了拟杆菌门的丰度,添加TP有助于肉鸡恢复肠道中厚壁菌门和拟杆菌门的比例,同时显著提高了肉鸡盲肠另枝菌属(Alistipes)和拟杆菌属(Bacteroides)的丰度。LPS刺激和日粮TP对提高肉鸡盲肠另枝菌属和降低肉鸡盲肠梭菌属UCG-014存在显著的交互作用。综上所述,茶多酚作为一种绿色饲料添加剂,可有效降低肉鸡肠道炎症指标,恢复肠道菌群微生态,促进肉鸡饲养产业健康发展。 展开更多
关键词 茶多酚 肉鸡 肠道炎症 肠道微生物
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