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1.
An efficient and rapid method to detect and verify natural antisense transcripts of animal genes
Zhang Li, Zhao Rui, Xiao Mei, Lin Shu-dai, Li Bi-xiao, Qiu Feng-fang, Ma Jing-e, Zhang Dexiang, Nie Qing-hua, An Li-long, Zhang Xi-quan
Journal of Integrative Agriculture 2016, 15 (
9
): 2070-2076. DOI:
10.1016/S2095-3119(15)61266-7
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1197
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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 lncRNA (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
(G elongation 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.
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2.
Research progress and strategies for multifunctional rapeseed: A case study of China
FU Dong-hui, JIANG Ling-yan, Annaliese S Mason, XIAO Mei-li, ZHU Long-rong, LI Li-zhi, ZHOU Qing-hong, SHEN Chang-jian, HUANG Chun-hui
Journal of Integrative Agriculture 2016, 15 (
8
): 1673-1684. DOI:
10.1016/S2095-3119(16)61384-9
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2063
)
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Rapeseed (
Brassica napus
), is an important source of edible oil, animal fodder, vegetables, condiments and biodiesel, and plays a significant role in securing edible oil production worldwide. However, in countries with comparatively low levels of agricultural mechanization, such as China, increasing costs of labor and agricultural inputs are decreasing rapeseed profitability, and hence the area of rapeseed under cultivation. If the value of rapeseed crops is not further increased, the rapeseed growing area will continue to decrease, potentially jeopardizing oil production. Therefore, full exploitation of the existing and potential value of rapeseed is desirable. Different rapeseed products are already utilized in different ways, with more applications currently underutilized. As well as oil extraction from the seeds, the shoot and leaves can be used as vegetables, the roots to absorb soil cadmium for pollution remediation, the flowers for sightseeing and as a source of nectar, the pollen for extracting flavonoids and useful amino acids, the seeds/seed meal for extracting isthiocyanates and other important sulforaphane compounds, the straw and seed meal for fodder, and immature whole plants for green manure. This review summarizes recent research on ways to explore the potential holistic value of rapeseed, by taking the example of multifunctionality of rapeseed in China.
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3.
Characterization of MicroRNA* Species in Peking Duck Skin
ZHANG Li, XIE Xiu-juan, JIA Shan-gang, XIAO Mei, LIN Shu-dai, AN Li-long, LUO Wen, JIA Xinzheng, NIE Qing-hua , ZHANG Xi-quan
Journal of Integrative Agriculture 2013, 12 (
9
): 1614-1619. DOI:
10.1016/s2095-3119(13)60494-3
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1285
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A substantial fraction of miRNA* species are conserved in animals and can repress activities of target genes. This study aims to investigate the miRNA* species in duck skin by using Solexa sequencing. We obtained a total of 96 miRNA* species in two skin small RNA libraries and identified 56 miRNA/miRNA* (miR/miR*) pairs. Nucleotide bias of miRNA* indicated that the priority was C>A>U>G for the first nucleotide and U>C>A>G for the last nucleotide. Comparison analyses showed that 3´-U accounted for a higher proportion in the 56 miR/miR* pairs. Among the top 20 expressed miRNA* species, 17 were shared by two libraries and most of the miRNA* species were highly conservative, especially in the “seed region”. miR-199a* were expressed highly in our samples, which was also previously shown abundant in mouse hair follicle. Furthermore, four miRNA* species were predicted to target their genes in signal pathways of feather follicle development and feather morphogenesis despite very low levels.
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