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2. Expression analysis and single-nucleotide polymorphisms of SYNDIG1L and UNC13C genes associated with thoracic vertebral numbers in sheep (Ovis aries)

Author

Ming-Xing Chu, Ran Di, Yingjie Zhong, Xiangyu Wang, Yang Yang, and Qiuyue Liu

Subjects
0301 basic medicine, Cultural Studies, biology, 0402 animal and dairy science, Religious studies, Adipose tissue, Single-nucleotide polymorphism, 04 agricultural and veterinary sciences, biology.organism_classification, 040201 dairy & animal science, Andrology, 03 medical and health sciences, 030104 developmental biology, Real-time polymerase chain reaction, Polymorphism (computer science), SNP, Ovis, Gene, Genetic association
Abstract

The objective of the current study was to analyze expression levels of synapse differentiation inducing 1-like (SYNDIG1L) and unc-13 homolog C (UNC13C) genes in different tissues, while single-nucleotide polymorphisms (SNPs) of two genes were associated with multiple thoracic vertebrae traits in both Small-tailed Han sheep (STH) and Sunite sheep (SNT). The expression levels of SYNDIG1L and UNC13C were analyzed in the brain, cerebellum, heart, liver, spleen, lung, kidney, adrenal gland, uterine horn, longissimus muscle, and abdominal adipose tissues of two sheep breeds with different thoracic vertebral number (TVN) sheep (T13 groups and T14 groups) by real-time quantitative polymerase chain reaction (RT-qPCR). Meanwhile, the polymorphisms of UNC13C gene g.52919279C>T and SYNDIG1L gene g.82573325C>A in T14 and T13 were genotyped by the Sequenom MassARRAY® SNP assay, and association analysis was performed with the TVN. The results demonstrated that UNC13C gene was extensively expressed in 11 tissues. The expression of UNC13C gene in longissimus muscle of T14 groups of STH was significantly higher than that of T13 groups (PA was significantly correlated with the TVN in both STH (P

Published
2021

3. Expression analysis of DIO2, EYA3, KISS1 and GPR54 genes in year-round estrous and seasonally estrous rams

Author

Qing Xia, Caihong Wei, Ming-Xing Chu, Xiaoyun He, and Ran Di

Subjects
0301 basic medicine, Cultural Studies, Estrous cycle, endocrine system, Cerebellum, Adrenal gland, Cerebrum, Religious studies, Vas deferens, DIO2, Biology, Epididymis, Andrology, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, medicine.anatomical_structure, Hypothalamus, medicine, hormones, hormone substitutes, and hormone antagonists, 030217 neurology & neurosurgery
Abstract

The expression characteristics of the hypothalamic–pituitary–gonadal (HPG) axis-related candidate genes, DIO2, EYA3, KISS1 and GPR54, were analyzed in year-round estrous rams (small-tail Han sheep, STH) and seasonally estrous rams (Sunite sheep, SNT) using qPCR. The results were as follows: DIO2 was mainly expressed in pituitary, and KISS1 was specifically expressed in hypothalamus in the two groups. However, EYA3 and GPR54 were widely expressed in the cerebrum, cerebellum, hypothalamus, pituitary, testis, epididymis, vas deferens and adrenal gland tissues in both breeds, with significant differences in the cerebellum, hypothalamus, pituitary, testis and vas deferens tissues. We speculated that DIO2 and KISS1 may have positive roles in different regions in ram year-round estrus. Moreover, the expression patterns of EYA3 and GPR54 suggested that they may regulate the estrous mode of ram via testis and vas deferens. This is the first study to systematically analyze the expression patterns of HPG axis-related genes in rams.

Published
2020

4. Genetic diversity estimation of Yunnan indigenous goat breeds using microsatellite markers

Author

Yuehui Ma, Guang-Xin E, Ming-Xing Chu, Yongju Zhao, Lan Zhu, Qiong-Hua Hong, and Yong-Fu Huang

Subjects
0106 biological sciences, China, microsatellite, Veterinary medicine, Population, Biology, 010603 evolutionary biology, 01 natural sciences, Indigenous, diversity, Loss of heterozygosity, 03 medical and health sciences, lcsh:QH540-549.5, Allele, education, Ecology, Evolution, Behavior and Systematics, Original Research, 030304 developmental biology, Nature and Landscape Conservation, 0303 health sciences, Genetic diversity, education.field_of_study, Ecology, Phylogenetic tree, Positive selection, Yunnan, indigenous goat, Microsatellite, lcsh:Ecology
Abstract

Background To assess the genetic diversity of seven Yunnan indigenous goat populations (Fengqing hornless goat, Mile red‐bone goat, Longling goat, Ninglang black goat, Black‐bone goat, Yunling black goat, and Zhaotong goat), their population structures were investigated using 20 microsatellite markers. Results The results indicated that the genetic diversity of these goats was rich. The observed heterozygosity ranged from 0.4667 ± 0.0243 to 0.5793 ± 0.0230, and the mean number of alleles ranged from 4.80 ± 1.61 and 4.80 ± 1.64 to 6.20 ± 2.93. The population structure analysis showed that these seven goat populations were separated into two clusters, consistent with the results from phylogenetic networks, pairwise differences, and STRUCTURE analyses. We speculate that this may have been caused by natural geographical isolation, human migration and economic and cultural exchanges. We suggest removing CSRD247 and ILSTS005, two loci identified to be under positive selection in the present study, from the microsatellite evaluation system of goats. Conclusions The present study may provide a scientific basis for the conservation and utilization of Yunnan indigenous goats.

Published
2019

5. Current genetic diversity in eight local Chinese sheep populations

Author

Guang-Xin E, Yuehui Ma, Qiong-Hua Hong, Ming-Xing Chu, and Yong-Fu Huang

Subjects
0301 basic medicine, China, Structure analysis, Population, Zoology, Breeding, Biology, 03 medical and health sciences, 0302 clinical medicine, Genetics, Animals, Allele, education, Molecular Biology, Phylogeny, education.field_of_study, Genetic diversity, Sheep, Phylogenetic tree, Genetic Variation, General Medicine, Breed, Genetic divergence, Genetics, Population, 030104 developmental biology, 030220 oncology & carcinogenesis, Microsatellite
Abstract

China has numerous local domestic sheep breeds. In this study, the genetic diversity of eight sheep populations was estimated using 17 microsatellites. Knowledge of such diversity provides novel insight into the degree of breed protection needed and the prediction of hybrid advantage. In total, 17 microsatellites were genotyped in 186 individuals from eight populations. The mean number of alleles (± SD) ranged from 3.71 ± 1.36 in Zhaotong sheep to 11.94 ± 3.58 in small-tailed Han sheep. The observed heterozygote frequency (± SD) within a population ranged from 0.482 ± 0.025 in Zhaotong sheep to 0.664 ± 0.023 in Tibetan sheep. In addition, using pairwise difference (FST) analysis, the highest within-population diversity was observed in Tibetan sheep (πX = 12.8098) and small-tailed Han (πX = 12.67873), and the lowest diversity was observed in Zhaotong sheep (πX = 7.90337). The results for genetic divergence between populations indicated that the populations were significantly different (P

Published
2018

6. The expression and mutation of

Author

Yu-Liang, Wen, Xiao-Fei, Guo, Lin, Ma, Xiao-Sheng, Zhang, Jin-Long, Zhang, Sheng-Guo, Zhao, and Ming-Xing, Chu

Subjects
endocrine system, Original Study
Abstract

Previous studies have shown that BMPR1B promotes follicular development and ovarian granulosa cell proliferation, thereby affecting ovulation in mammals. In this study, the expression and polymorphism of the BMPR1B gene associated with litter size in small-tail Han (STH) sheep were determined. The expression of BMPR1B was detected in 14 tissues of STH sheep during the follicular phase as well as in the hypothalamic–pituitary–gonadal (HPG) axis of monotocous and polytocous STH sheep during the follicular and luteal phases using quantitative polymerase chain reaction (qPCR). Sequenom MassARRAY® single nucleotide polymorphism (SNP) technology was also used to detect the polymorphism of SNPs in seven sheep breeds. Here, BMPR1B was highly expressed in hypothalamus, ovary, uterus, and oviduct tissue during the follicular phase, and BMPR1B was expressed significantly more in the hypothalamus of polytocous ewes than in monotocous ewes during both the follicular and luteal phases (PG locus had significant negative effects on the litter size of STH sheep, and the combination of g.29380965A>G and FecB (Fec – fecundity and B – Booroola; A746G) at the BMPR1B gene showed that the litter size of AG–GG, AA–GG, and GG–GG genotypes was significantly higher compared with other genotypes (P

Published
2020

7. Expression analysis and single-nucleotide polymorphisms of

Author

Ying-Jie, Zhong, Yang, Yang, Xiang-Yu, Wang, Ran, Di, Ming-Xing, Chu, and Qiu-Yue, Liu

Subjects
Original Study
Abstract

The objective of the current study was to analyze expression levels of synapse differentiation inducing 1-like (SYNDIG1L) and unc-13 homolog C (UNC13C) genes in different tissues, while single-nucleotide polymorphisms (SNPs) of two genes were associated with multiple thoracic vertebrae traits in both Small-tailed Han sheep (STH) and Sunite sheep (SNT). The expression levels of SYNDIG1L and UNC13C were analyzed in the brain, cerebellum, heart, liver, spleen, lung, kidney, adrenal gland, uterine horn, longissimus muscle, and abdominal adipose tissues of two sheep breeds with different thoracic vertebral number (TVN) sheep (T13 groups and T14 groups) by real-time quantitative polymerase chain reaction (RT-qPCR). Meanwhile, the polymorphisms of UNC13C gene g.52919279C>T and SYNDIG1L gene g.82573325C>A in T14 and T13 were genotyped by the Sequenom MassARRAY® SNP assay, and association analysis was performed with the TVN. The results demonstrated that UNC13C gene was extensively expressed in 11 tissues. The expression of UNC13C gene in longissimus muscle of T14 groups of STH was significantly higher than that of T13 groups (PA was significantly correlated with the TVN in both STH (P

Published
2020

8. Evolutionary relationship and population structure of domestic Bovidae animals based on MHC-linked and neutral autosomal microsatellite markers

Author

Jian-Lin Han, Yong-Fu Huang, Wang-Dui Basang, Zhong-Quan Zhao, Ming-Xing Chu, Yan Zeng, Guang-Xin E, Bai-Gao Yang, Qiong-Hua Hong, Jia-Hua Zhang, Yan-Guo Han, Dong-Ke Zhou, Yongju Zhao, Yan-Bin Zhu, Yuehui Ma, Li-Peng Chen, Lu-Pei Zhang, and Ri-Su Na

Subjects
0301 basic medicine, Heterozygote, Immunology, Population, Major histocompatibility complex, Analysis of molecular variance, Loss of heterozygosity, Major Histocompatibility Complex, 03 medical and health sciences, 0302 clinical medicine, Animals, education, Molecular Biology, Phylogeny, education.field_of_study, biology, Haplotype, Genetic Variation, Phylogenetic network, Biological Evolution, 030104 developmental biology, Haplotypes, Evolutionary biology, Phylogenetic Pattern, Animals, Domestic, Host-Pathogen Interactions, biology.protein, Microsatellite, Cattle, 030215 immunology, Microsatellite Repeats
Abstract

Major histocompatibility complex (MHC) genes are critical for disease resistance or susceptibility responsible for host-pathogen interactions determined mainly by extensive polymorphisms in the MHC genes. Here, we examined the diversity and phylogenetic pattern of MHC haplotypes reconstructed using three MHC-linked microsatellite markers in 55 populations of five Bovidae species and compared them with those based on neutral autosomal microsatellite markers (NAMs). Three-hundred-and-forty MHC haplotypes were identified in 1453 Bovidae individuals, suggesting significantly higher polymorphism and heterozygosity compared with those based on NAMs. The ambitious boundaries in population differentiation (phylogenetic network, pairwise FST and STRUCTURE analyses) within and between species assessed using the MHC haplotypes were different from those revealed by NAMs associated closely with speciation, geographical distribution, domestication and management histories. In addition, the mean FST was significantly correlated negatively with the number of observed alleles (NA), observed (HO) and expected (HE) heterozygosity and polymorphism information content (PIC) (P 0.05) between the MHC haplotype and NAMs datasets. Analysis of molecular variance (AMOVA) revealed a lower percentage of total variance (PTV) between species/groups based on the MHC-linked microsatellites than NAMs. Therefore, it was inferred that individuals within populations accumulated as many MHC variants as possible to increase their heterozygosity and thus the survival rate of their affiliated populations and species, which eventually reduced population differentiation and thereby complicated their classification and phylogenetic relationship inference. In summary, host-pathogen coevolution and heterozygote advantage, rather than demographic history, act as key driving forces shaping the MHC diversity within the populations and determining the interspecific MHC diversity.

Published
2019

9. Gene Expression and Localization of LAMTOR3 in the Skin Cells of Liaoning Cashmere Goats

Author

Jing'ai Piao, Xu Guo, Jun Piao, Fengqin Zhao, Ming Cao, Mei Jin, and Ming-xing Chu

Subjects
Male, 0301 basic medicine, MAPK/ERK pathway, MAP Kinase Signaling System, Endosome, Bioengineering, Biology, Melatonin, 03 medical and health sciences, Genetic resources, Gene expression, medicine, Animals, Insulin-Like Growth Factor I, Noggin, Protein kinase A, Adaptor Proteins, Signal Transducing, Skin, integumentary system, Goats, 0402 animal and dairy science, 04 agricultural and veterinary sciences, 040201 dairy & animal science, Cell biology, 030104 developmental biology, Gene Expression Regulation, Female, Animal Science and Zoology, Carrier Proteins, Hair Follicle, Biotechnology, medicine.drug
Abstract

Liaoning cashmere goats are the most precious genetic resources in China. The function of LAMTOR3 [late endosomal/lysosomal adaptor, mitogen-activated protein kinase (MAPK), and mammalian target of rapamycin activator 3/MAPK scaffold protein 1] gene is expressed in the skin of Liaoning cashmere goats. In situ hybridization (ISH) found that LAMTOR3 is expressed in the inner root sheath (IRS) of hair follicles. During the anagen or catagen phase, the expression of LAMTOR3 is higher in secondary hair follicles than in primary hair follicles. Expression of LAMTOR3 in skin cells treated with melatonin or insulin-like growth factor-1 (IGF-1) is lower than in untreated cells. In addition, the simultaneous treatment of fibroblast growth factor 5 and melatonin decrease the expression of LAMTOR3 in skin cells. The simultaneous treatment with melatonin and 10−5 g/L IGF-1 or 10−4 g/L IGF-1 increases the expression of LAMTOR3 gene in skin cells. If Noggin expression is decreased, then LAMTOR3 expression is increased. This hypothesis suggested that LAMTOR3 influences the character of cashmere fiber, and it may regulate the development of hair follicle and cashmere growth by inducing the MAPK signaling pathway.

Published
2018

10. Construction and expression of a prokaryotic expression vector for the goat sry gene

Author

Wei-Wei Ni, Yong-Fu Huang, Shu-Zhu Cheng, Guang-Xin E, Xiao Wang, Yue-Hui Ma, and Ming-Xing Chu

Subjects
Expression vector, General Veterinary, Cloning vector, lac operon, Biology, medicine.disease_cause, Molecular biology, law.invention, Restriction enzyme, Plasmid, Testis determining factor, law, medicine, Recombinant DNA, Animal Science and Zoology, Escherichia coli
Abstract

Goats are economically important animals in the world, and their sex is an important factor in their economic efficiency. Reconstruction of a goat SRY gene expression vector can lay a foundation for studying the immunogenicity and sex determination of SRY protein at the molecular level. In this study, the coding region of the goat SRY gene was used as the target gene fragment for synthesis and optimization, and the cloning vector was used as a template to amplify the target gene and finally ligated to the expression vector pET-SUMO. The recombinant plasmid was then verified by the double restriction enzyme method and transformed into Escherichia coli (DE3). After the induction of expression by Isopropyl â-D-Thiogalactoside (IPTG), the cells were lysed, and SDS-PAGE electrophoresis was performed to observe the expression of the recombinant protein. Additionally, the immunological activity of the recombinant protein was assessed. The target gene was successfully ligated into the prokaryotic expression vector pET-28a; additionally, the prokaryotic expression plasmid pET-SUMO was successfully constructed, and the SRY antigen protein (42 kDa) was expressed. The titer of the rabbit antiserum (PAI-1608012-1) was more than 1:50000, as measured by ELISA, which demonstrated that the titer and the sensitivity of the rabbit serum reached the expected levels. In this study, the prokaryotic expression vector pET-SUMO was successfully constructed. The recombinant protein has high immunopotency and immunoreactivity, which lays a foundation for the preparation of antibodies and the molecular sexing of goats in the future.

Published
2019

11. [Comparison of different single cell whole genome amplification methods and MALBAC applications in assisted reproduction]

Author

Ya Xin, Yao, Yong Fu, La, Ran, Di, Qiu Yue, Liu, Wen Ping, Hu, Xiang Yu, Wang, and Ming Xing, Chu

Subjects
Reproductive Techniques, Assisted, Reproduction, Animals, Humans, DNA, Genomics, Single-Cell Analysis, Nucleic Acid Amplification Techniques
Abstract

Single-cell whole genome amplification (WGA) is a new technology, which can amplify small amounts of DNA from single cell and obtain the high coverage whole genome DNA template for revealing cell heterogeneity. Single cell WGA methods mainly include primer extension preamplification PCR (PEP-PCR), degenerate oligonucleotide primed PCR (DOP-PCR), multiple displacement amplification (MDA), and multiple annealing and looping-based amplification cycles (MALBAC). In this review, we describe the principles and applications of different single cell genome wide amplification, and we evaluate and compare their amplification efficiency, including the coverage of genome, homogeneity, reproducibility, and detection power of single-nucleotide variants (SNV) and copy number variants (CNV). The results show that MALBAC have the highest amplification homogeneity, the lowest allelic gene knockdown rate, the best reproducibility, and the best detection effect on CNV and SNV. We also describe the applications of MALBAC in human single sperm meiosis, aneuploidy analysis, and human oocyte genome research.

Published
2018

12. [The molecular mechanism of sheep seasonal breeding and artificial regulatory techniques for estrus and mating in anestrus]

Author

Qing, Xia, Qiu Yue, Liu, Xiang Yu, Wang, Wen Ping, Hu, Chun Yan, Li, Xiao Yun, He, Ming Xing, Chu, and Ran, Di

Subjects
Male, Sheep, Estrus, Animals, Female, Seasons, Breeding, Anestrus
Abstract

Seasonal breeding is an important factor limiting sheep production efficiency. Detailed analysis on the molecular mechanisms of seasonal breeding is the premise for improving estrus and mating rate of sheep during anestrus. Recent research showed that under long-photoperiod and short-photoperiod conditions, a series of changes in signaling molecules and cell morphology could be observed in ovine seasonal reproduction pathway. Based on the molecular mechanisms of seasonal reproduction, several technologies or methods for inducing estrus and mating of ewes in anestrus have been developed. In this review, photoperiod-induced changes in signaling molecules and cell morphology in pituitary and hypothalamic tissue are first summarized in terms of the molecular mechanisms and characteristics of seasonal reproduction. The application effect, advantages and disadvantages for applying these technologies for inducing estrus and mating of ewes in anestrus are then discussed, thereby providing the critical insights in identifying a new technology, which is environmentally friendly and efficient, to improve breeding rate in anestrus.

Published
2018

13. Genetic diversity of the Chinese goat in the littoral zone of the Yangtze River as assessed by microsatellite and mtDNA

Author

Lan Zhu, Yuehui Ma, Yong-Fu Huang, Hui-Jiang Gao, Yan-Guo Han, Qiong-Hua Hong, Jia-Hua Zhang, Yongju Zhao, Li-Peng Chen, Gaofu Wang, Lanhui Li, Yuan-Zhi Sun, Guang-Xin E, Mei-Lan Jin, Xiang-Long Li, Ji-Jun Guo, Zhou Peng, Huai-Zhi Jiang, Ming-Xing Chu, Cao-De Jiang, and Ren Hangxing

Subjects
0301 basic medicine, Genetic diversity, microsatellite, Lineage (genetic), Yangtze River, Ecology, Phylogenetic tree, Haplotype, goat, 0402 animal and dairy science, Population genetics, 04 agricultural and veterinary sciences, mitochondrial DNA, Biology, 040201 dairy & animal science, diversity, 03 medical and health sciences, 030104 developmental biology, Evolutionary biology, Phylogenetics, Microsatellite, Genetic variability, Ecology, Evolution, Behavior and Systematics, Nature and Landscape Conservation, Original Research
Abstract

The objective of this study was to assess the genetic diversity and population structure of goats in the Yangtze River region using microsatellite and mtDNA to better understand the current status of those goat genetic diversity and the effects of natural landscape in fashion of domestic animal genetic diversity. The genetic variability of 16 goat populations in the littoral zone of the Yangtze River was estimated using 21 autosomal microsatellites, which revealed high diversity and genetic population clustering with a dispersed geographical distribution. A phylogenetic analysis of the mitochondrial D‐loop region (482 bp) was conducted in 494 goats from the Yangtze River region. In total, 117 SNPs were reconstructed, and 173 haplotypes were identified, 94.5% of which belonged to lineages A and B. Lineages C, D, and G had lower frequencies (5.2%), and lineage F haplotypes were undetected. Several high‐frequency haplotypes were shared by different ecogeographically distributed populations, and the close phylogenetic relationships among certain low‐frequency haplotypes indicated the historical exchange of genetic material among these populations. In particular, the lineage G haplotype suggests that some west Asian goat genetic material may have been transferred to China via Muslim migration.

Published
2017

14. Identification of Differentially Expressed Long Noncoding RNAs and mRNAs Involved with Dominant Follicle Selection in Goats using RNA-seq

Author

Wang-Dui Basang, Di Liu, Jia-Hua Zhang, Yan-Bin Zhu, Li Liu, Xiao-Lin Luo, Guang-Xin E, Yongju Zhao, Shi-Cheng He, Huai-Zhi Jiang, Ming-Xing Chu, Yong-Fu Huang, Tian-Wu An, Zhong-Quan Zhao, Yue-Hui Ma Ma, Hui-Jiang Gao, and Luobu Danjiu

Subjects
Dominant follicle, Animal Science and Zoology, Identification (biology), RNA-Seq, Computational biology, Biology, Selection (genetic algorithm)
Published
2017

15. Screening for S32G mutation of BMP15 gene in 18 goat breeds

Author

Tao FENG, Ming-Xing CHU, Gui-Ling CAO, Dong-Wei HUANG, Ran DI, Qiu-Yue LIU, Zhang-Yuan PAN, Mei JIN, and Ying-Jie ZHANG

Subjects
Genetics, Litter (animal), genomic DNA, General Veterinary, Goat,prolificacy,bone morphogenetic protein 15 gene,functional analysis, Mutation (genetic algorithm), Genetic structure, Allele, Biology, Fecundity, Gene, Breed
Abstract

In our early work, one mutation (A898G, which caused Ser32Gly (S32G) change of mature peptide) was identified in the goat BMP15 gene and the allele G was associated with high litter size in Jining Grey goats (the goat breed with the highest fecundity in China). The aim of this research was to investigate the genetic structure of the prolific BMP15 gene in 18 goat breeds reared in China, including 12 native breeds, 3 introduced breeds, and 2 cultivated breeds. Genomic DNA of 1011 goats was screened for the S32G mutation. The results showed that this mutation existed in all 3 cultivated and 8 native goat breeds but in none of the 3 introduced goat breeds, which hinted that this mutation may originate from native goat breeds of China. Besides the Jining Grey goats, the BMP15 gene was also a potential prolificacy gene in Matou goats. Moreover, the structure prediction indicated that the S32G mutation might participate in the binding of BMP15 with receptors.

Published
2014

16. Expression of the GPRC5D gene in Liaoning Cashmere goats

Author

Jing'ai Piao, Mei Jin, YangLe Qu, YiMeng Wang, Ming-xing Chu, XiuNa Li, and Jun Piao

Subjects
Transmembrane domain, Real-time polymerase chain reaction, integumentary system, General Veterinary, Bioinformatics analysis, Cashmere goat, GPRC5D gene, GPRC5D,bioinformatics,RT-PCR,in situ hybridization, In situ hybridization, Biology, Inner root sheath, Molecular biology
Abstract

This study aimed to characterize the expression the GPRC5D gene in the skin of the Liaoning Cashmere goat. Initially, the GPRC5D gene sequence was subjected to bioinformatics analysis. Second, semiquantitative RT-PCR was used to detect GPRC5D gene expression in the tissues. Third, in situ hybridization was used to locate GPRC5D gene expression in the primary and secondary hair follicles. Functional site analysis showed that GPRC5D has 7 transmembrane domains. RT-PCR showed that GPRC5D was expressed only in the skin. In situ hybridization showed that GPRC5D was expressed in the inner root sheath only. We speculated that GPRC5D may regulate cashmere growth.

Published
2014

17. Selection signature in domesticated animals

Author

Zhang-yuan, Pan, Xiao-yun, He, Xiang-yu, Wang, Xiao-fei, Guo, Xiao-han, Cao, Wen-ping, Hu, Ran, Di, Qiu-yue, Liu, and Ming-xing, Chu

Subjects
Dogs, Sheep, Swine, Animals, Domestic, Animals, Cattle, Selection, Genetic
Abstract

Domesticated animals play an important role in the life of humanity. All these domesticated animals undergo same process, first domesticated from wild animals, then after long time natural and artificial selection, formed various breeds that adapted to the local environment and human needs. In this process, domestication, natural and artificial selection will leave the selection signal in the genome. The research on these selection signals can find functional genes directly, is one of the most important strategies in screening functional genes. The current studies of selection signal have been performed in pigs, chickens, cattle, sheep, goats, dogs and other domestic animals, and found a great deal of functional genes. This paper provided an overview of the types and the detected methods of selection signal, and outlined researches of selection signal in domestic animals, and discussed the key issues in selection signal analysis and its prospects.

Published
2016

18. Application of epigenetic markers in molecular breeding of the swine

Author

Ke, Zhang, Guang-de, Feng, Bao-yun, Zhang, Wei, Xiang, Long, Chen, Fang, Yang, Ming-xing, Chu, and Ping-qing, Wang

Subjects
Swine, Animals, Breeding, DNA Methylation, Biomarkers, Epigenesis, Genetic
Abstract

Livestock phenotypes are determined by the interaction of a variety of factors, including the genome, the epigenome and the environment. Epigenetics refers to gene expression changes without DNA sequence alterations. Epigenetic markers mainly include DNA methylation, histone modifications, non-coding RNAs, and imprinting genes. More and more researches show that epigenetic markers play an important role in the traits of pigs by modulating phenotype changes via gene expression. However, the role of epigenetic markers has caught little attention in swine breeding. The mechanism that influences important traits of swine has not been analyzed in detail, and it still lacks adequate scientific basis for practical applications. From the aspects of nutrition, diseases, important economic traits and trans-generational inheritance, we summarize the research, application prospects and challenges in the field of utilizing epigenetic markers in molecular breeding of pigs, thus providing a more comprehensive theoretical basis to promote more rapid research development in this field.

Published
2016

19. [A mechanistic review of how hypoxic mircroenvironment regulates mammalian ovulation]

Author

Fang, Yang, Bao-yun, Zhang, Guang-de, Feng, Wei, Xiang, Yun-xia, Ma, Hang, Chen, Ming-xing, Chu, and Ping-qing, Wang

Subjects
Mammals, Ovulation, Vascular Endothelial Growth Factor A, Cellular Microenvironment, Ovarian Follicle, Animals, Humans, Female, Hypoxia-Inducible Factor 1, Hypoxia
Abstract

Mammalian ovulation is a complicated process that includes development of follicles, ovulation, formation of corpus luteum and luteolysis. The three different stages of the ovulation activity are affected by hypoxic microenvironment and hypoxia-induced factors (HIF), which play a crucial role in physiologyical processes, such as angiogenesis and inflammation. Although the process of ovulation has been well elucidated, the molecular mechanism regulated by hypoxia needs an in depth study. In this review, we summarize how hypoxic and HIF regulate gene expression during mammalian ovulation in order to provide a better understanding of ovulation mechanism, which may lay a theoretical basis for prevention and therapy of various ovarian diseases.

Published
2016

20. [The mechanism of miRNA-mediated PGR signaling pathway in regulating female reproduction]

Author

Long, Chen, Bao-yun, Zhang, Guang-de, Feng, Wei, Xiang, Yun-xia, Ma, Hang, Chen, Ming-xing, Chu, and Ping-qing, Wang

Subjects
MicroRNAs, Reproduction, Animals, Humans, Female, Receptors, Progesterone, Progesterone, Signal Transduction
Abstract

MicroRNAs (miRNAs) are involved in several physiological processes as important post-transcriptional regulators. Progesterone (P4), an important steroid hormone, produces physiological effect through binding specific receptor progesterone receptors (PGR) which regulates functions of both reproductive and non-reproductive tissues as a member of the nuclear receptor superfamily. P4/PGR and miRNAs could regulate female reproduction independently, however, it is still unclear how miRNAs and P4/PGR interaction regulates female reproductive activities such as ovulation in female reproduction. In this review, we summarize the possible ways in which miRNAs regulate P4 production and PGR gene expression as well as P4/PGR regulate miRNAs expression, which provide a theoretical basis for further studying the role of miRNAs and P4/PGR in female reproduction.

Published
2016

21. Research progress in molecular mechanism of animal seasonal reproduction

Author

Dong-Wei Huang and Ming-Xing Chu

Subjects
photoperiodism, endocrine system, medicine.medical_specialty, Gnrh secretion, media_common.quotation_subject, General Medicine, Biology, Melatonin, Endocrinology, Gonadal Steroid Hormones, Internal medicine, medicine, Molecular mechanism, Secretion, Hormone metabolism, Reproduction, hormones, hormone substitutes, and hormone antagonists, media_common, medicine.drug
Abstract

Animal seasonal reproduction involves complicated neuroendocrine processes of the hypothalamo-pituitary-gonadal axis. It is dominantly regulated by photoperiod, a crucial environmental cue. Melatonin, as internal photoperiod signal, regulates seasonal reproduction of animals. In recent years, it has been found that Kiss1/GPR54 system, which may influence GnRH secretion evidently, is regulated by both melatonin and feedback action of gonadal steroid hormones. Consequently, Kiss1/GPR54 system may play a key role in seasonal reproduction. Additionally, there exists another potential retrograde control pathway of seasonal breeding, which involves TSH-DIO2/DIO3 system. TSH-DIO2/ DIO3 system affects synthesis and secretion of GnRH and is regulated by melatonin, as well as Kiss1/GPR54 system. In this article, melatonin signal, especially the research advances of Kissl/GPR54 system and TSH-DIO2/DIO3 system were reviewed.

Published
2011

22. Soft contact lens biosensor for in situ monitoring of tear glucose as non-invasive blood sugar assessment

Author

Kenji Sano, Yasuhiko Iwasaki, Kumiko Miyajima, Daishi Takahashi, Shin-ichi Sawada, Hiroyuki Kudo, Manabu Mochizuki, Kohji Mitsubayashi, Takahiro Arakawa, Kazunari Akiyoshi, and Ming Xing Chu

Subjects
Blood Glucose, Auxiliary electrode, Working electrode, Chromatography, biology, Chemistry, technology, industry, and agriculture, Analytical chemistry, Blood sugar, Biosensing Techniques, macromolecular substances, Contact Lenses, Hydrophilic, Analytical Chemistry, Contact lens, Basal (medicine), Tears, Electrode, biology.protein, Animals, Humans, Glucose oxidase, Rabbits, sense organs, Biosensor
Abstract

A contact lens (CL) biosensor for in situ monitoring of tear glucose was fabricated and tested. Biocompatible 2-methacryloyloxyethyl phosphorylcholine (MPC) polymer and polydimethyl siloxane (PDMS) were employed as the biosensor material. The biosensor consists of a flexible Pt working electrode and a Ag/AgCl reference/counter electrode, which were formed by micro-electro-mechanical systems (MEMS) technique. The electrode at the sensing region was modified with glucose oxidase (GOD). The CL biosensor showed a good relationship between the output current and glucose concentration in a range of 0.03-5.0mM, with a correlation coefficient of 0.999. The calibration range covered the reported tear glucose concentrations in normal and diabetic patients. Also, the CL biosensor was applied to a rabbit for the purpose of tear glucose monitoring. The basal tear glucose was estimated to 0.11 mM. Also, the change of tear glucose induced by the change of blood sugar level was assessed by the oral glucose tolerance test. As a result, tear glucose level increased with a delay of 10 min from blood sugar level. The result showed that the CL biosensor is expected to provide further detailed information about the relationship between dynamics of blood glucose and tear glucose.

Published
2011

23. TWO EXTREME X-RAY MUTATIONS OF MORPHOLOGICAL INTEREST

Author

Ming-Xing Chu, Xiao-Hong Guo, and Zhong-Xiao Zhou

Subjects
Regulation of gene expression, genetic structures, Protein family, RNA, Kidney metabolism, General Medicine, Biology, Cell biology, Retinol binding protein, Botany, Genetics, Receptor, Gene, Function (biology)
Abstract

Retinol-binding proteins (RBPs) are a kind of circulating carrier proteins for serum and cellular retinol and retinol acid, which are lipid-soluble vitamins, and are members of hydrophobic binding protein family. Serum RBPs were synthesized primarily in liver, then was released into blood streams, and then to various tissues. Under the interaction with substances such as retinol, pre-albumin and the receptors of cellular surface, they play important roles in storage, metabolism of VitA and transport of VitA to the target cells. Cellular RBPs play the similar function as serum RBPs in intracell. This review introduces action mechanism, tissue localization and developmental expression of retinol-binding proteins. This review also introduces the structure, chromosome mapping and their relationships with reproductive performance of retinol-binding protein genes.

Published
2010

24. A soft and flexible biosensor using a phospholipid polymer for continuous glucose monitoring

Author

Ming Xing Chu, Kazunari Akiyoshi, Yasuhiko Iwasaki, Kohji Mitsubayashi, Kumiko Miyajima, Hirokazu Saito, Nobuyuki Morimoto, Hiroyuki Kudo, Takayuki Shirai, and Kazuyoshi Yano

Subjects
Materials science, Phosphorylcholine, Biomedical Engineering, Phospholipid, Analytical chemistry, Biosensing Techniques, Sensitivity and Specificity, Glucose Oxidase, chemistry.chemical_compound, Humans, Glucose oxidase, Pliability, Hydrogen peroxide, Polytetrafluoroethylene, Molecular Biology, chemistry.chemical_classification, Chromatography, biology, technology, industry, and agriculture, Membranes, Artificial, Polymer, Enzymes, Immobilized, Amperometry, Glucose, Membrane, chemistry, Electrode, biology.protein, Methacrylates, Biosensor
Abstract

A flexible biosensor using a phospholipid polymer to immobilization of glucose oxidase (GOD) was fabricated and tested. At first, an enzyme membrane formed by immobilizing GOD onto a porous polytetrafluoroethylene (PTFE) membrane using the phospholipid polymer (2-methacryloyloxyethyl phosphorylcholine (MPC) copolymerized with 2-ethylhexylmethacrylate (EHMA):PMEH) was evaluated. According to the result of amperometric measurement, average density of GOD to be immobilized was optimized to 38.9 units cm(-2). Temperature and pH dependences were also investigated. Then, a flexible glucose sensor was fabricated by immobilizing GOD onto a flexible hydrogen peroxide electrode using PMEH. The flexible glucose sensor showed a linear relationship between output currents and glucose concentration in 0.05-1.00 mmol L(-1), with a correlation coefficient of 0.999. The calibration range covered the normal tear glucose level of 0.14-0.23 mmol L(-1). This indicates that the flexible biosensor is considered to be useful for monitoring of glucose in tear fluids.

Published
2009

25. Identification and verification of differentially expressed genes in the caprine hypothalamic-pituitary-gonadal axis that are associated with litter size

Author

Tao, Feng, Gui-Ling, Cao, Ming-Xing, Chu, Ran, Di, Dong-Wei, Huang, Qiu-Yue, Liu, Zhang-Yuan, Pan, Mei, Jin, Ying-Jie, Zhang, and Ning, Li

Subjects
China, Hypothalamo-Hypophyseal System, Multifactorial Inheritance, Base Sequence, Litter Size, Subtractive Hybridization Techniques, Goats, Molecular Sequence Data, Gene Expression Regulation, Developmental, Sequence Analysis, DNA, Breeding, Real-Time Polymerase Chain Reaction, Pregnancy, Animals, Female, Gonads, DNA Primers, Gene Library
Abstract

Litter size is a favorable economic trait for the goat industry, but remains a complex trait controlled by multiple genes in multiple organs. Several genes have been identified that may affect embryo survival, follicular development, and the health of fetuses during pregnancy. Jining Grey goats demonstrate the largest litter size among goat breeds indigenous to China. In order to better understand the genetic basis of this trait, six suppression subtractive hybridization (SSH) cDNA libraries were constructed using pooled mRNAs from hypothalamuses, pituitaries, and ovaries of sexually mature and adult polytocous Jining Grey goats, as testers, versus the pooled corresponding mRNAs of monotocous Liaoning Cashmere goats, as drivers. A total of 1,458 true-positive clones--including 955 known genes and 481 known and 22 unknown expressed sequence tags--were obtained from the SSH libraries by sequencing and alignment. The known genes were categorized into cellular processes and signaling information storage and processing, and metabolism. Three genes (FTH1, GH, and SAA) were selected to validate the SSH results by quantitative real-time PCR; all three were up-regulated in the corresponding tissues in the tester group indicating that these are candidate genes associated with the large litter size of Jining Grey goats. Several other identified genes may affect embryo survival, follicular development, and health during pregnancy. This study provides insights into the mechanistic basis by which the caprine hypothalamic-pituitary-gonadal axis affects reproductive traits and provides a theoretical basis for goat production and breeding.

Published
2014

26. The Study on Biological Function of Keratin 26, a Novel Member of Liaoning Cashmere Goat Keratin Gene Family

Author

Jun Piao, Jing Wang, Fengqin Zhao, Ming-xing Chu, Mei Jin, and Jing'ai Piao

Subjects
0301 basic medicine, Cell signaling, Hair Growth, Physiology, lcsh:Medicine, Signal transduction, Biochemistry, 0302 clinical medicine, Animal Cells, Keratin, Medicine and Health Sciences, Cashmere goat, lcsh:Science, BMP signaling pathway, Skin, Connective Tissue Cells, Mammals, chemistry.chemical_classification, Regulation of gene expression, Multidisciplinary, integumentary system, Goats, Wool, Telogen Phase, Ruminants, Anatomy, Cell biology, medicine.anatomical_structure, Connective Tissue, 030220 oncology & carcinogenesis, Vertebrates, Keratins, Folliculogenesis, Integumentary System, Cellular Types, Hair Follicle, Research Article, BMP signaling, macromolecular substances, Root sheath, 03 medical and health sciences, Hair Follicles, medicine, Animals, Catagen Phase, Noggin, lcsh:R, Anagen Phase, Organisms, Biology and Life Sciences, Proteins, Fibroblasts, Hair follicle, Cytoskeletal Proteins, Biological Tissue, 030104 developmental biology, Gene Expression Regulation, chemistry, Amniotes, lcsh:Q, Physiological Processes, Hair
Abstract

In our research, we explored the relationship between Keratin 26 and the regulation of fine hair, BMP signaling pathway, MT, FGF5, and IGF-I. The result of hybridization in situ revealed that Keratin 26 was specially expressed in cortex of skin hair follicles; the result of immunohistochemistry indicated that Keratin 26 was expressed in internal root sheath, external root sheath. Then, Real-time quantitative PCR results showed that relative expressive quantity of Keratin 26 was 1.08 or 3.3 × greater in secondary follicle than primary follicle during anagen or catagen; the difference during anagen was not remarkable (p>0.05), however, that of catagen was extremely significant (p

Published
2016

27. [Effects of RFRP-3 on reproductive function and energy balance in mammals]

Author

Wei, Xiang, Ping, Lai, Bao-Yun, Zhang, Ping-Qing, Wang, Ming-Xing, Chu, Qi, Fan, Chong-Xu, Liu, and Ying, Tan

Subjects
Mammals, Hypothalamo-Hypophyseal System, Reproduction, Neuropeptides, Animals, Pituitary-Adrenal System, Energy Metabolism
Abstract

The hypothalamo-pituitary-gonadal (HPG) axis integrates internal and external cues via a balance of stimulatory and inhibitory neurochemical systems to regulate reproductive function in mammals. However, RFRP-3 is a unique inhibitor of HPG axis at the hypothalamuic level in mammals to date. A large number of previous studies have confirmed that RFamide-related peptide (RFRP-3) suppresses gonadotropin-releasing hormone (GnRH) system and luteinizing hormone (LH) secretion, thereby affecting the reproduction. However, whether the inhibition of LH secretion by RFRP-3 occurs at the pituitary level or the hypothalamus level is not clear. It is interesting that RFRP-3 is also related to signal pathway of melatonin modulating mammal seasonal reproduction, but little is known about the effects of melatonin on the RFRP-3 neuron up to now. In addition, RFRP-3 also plays an important role in the regulation of energy balance and behavior. The regulatory mechanism of RFRP-3 in HPG axis and role of RFRP-3 in modulating mammalian energy balance, as well as behavior, are systematically elaborated and the remaining unsolved problems are also discussed in this paper.

Published
2012

28. [The neuroendocrine regulatory mechanisms of mammalian seasonal reproduction]

Author

Ping, Lai, Ping-Qing, Wang, Bao-Yun, Zhang, Ming-Xing, Chu, Chong-Xu, Liu, Ying, Tan, and Qi, Fan

Subjects
Mammals, Reproduction, Animals, Humans, Seasons, Breeding, Neurosecretory Systems, Signal Transduction
Abstract

The seasonal reproduction of mammal means the reproduction experiences an annual period from quiescence to renaissance. Studies have shown that kisspeptin and RFRP play an important role in the reproductive seasonality. The non-breeding season is characterized by an increase in the negative feedback effect of estrogen on GnRH, and this effect is transmitted by kisspeptin neurons, which may be an important factor affecting the reproduction activities. The expression of RFRP depends on melatonin secretion, and shows an apparent inhibition on reproduction in non-breeding season. In addition, thyroid hormones influence termination of the breeding season. Dopaminergic neuron A14/A15 also contributes to the seasonal changes in estrogen negative feedback. These neural systems may synergistically modulate the seasonal changes of reproductive function with the photoperiod. This review makes a systematic expatiation on the relationship between seasonal reproduction and these neural systems.

Published
2012

29. [Polymorphic and linkage analysis of microsatellite BMS2508 and FecB gene in sheep]

Author

Yan-Lu, Li, Ming-Xing, Chu, Hong-Quan, Chen, Li, Fang, Ran, DI, Yue-Hui, Ma, and Kui, Li

Subjects
Fertility, Polymorphism, Genetic, Sheep, Genetic Linkage, Animals, Genetic Variation, Ion Pumps, Linkage Disequilibrium, Microsatellite Repeats
Abstract

Genetic polymorphisms of microsatellite locus BMS2508, which was closely linked to the ovine fecundity gene FecB, were detected in prolific (Small Tail Han sheep) and non-prolific breeds of sheep (Texel, Dorset and Chinese Merino). The linkage disequilibrium between microsatellite locus BMS2508 and FecB gene of Small Tail Han sheep was also analyzed. There was the same mutation (A746G) of BMPR-IB gene in Small Tail Han sheep as that of FecB in Booroola Merino ewes, but the FecB mutation was absent in Texel, Dorset and Chinese Merino sheep. The genotype frequencies of BB, B+ and ++ were 0.485, 0.398 and 0.117 in Small Tail Han sheep, respectively. There were eight alleles varied from 94 bp to 116 bp and 15 genotypes detected at BMS2508 locus in four sheep breeds totally 438 individual. The preponderant allele was 100 bp, 94 bp, 94 bp, 112 bp, 100 bp, 100 bp, 112 bp, and the frequency was 0.453, 0.544, 0.802, 0.475, 0.483, 0.439, 0.389 in Small Tail Han (n=307), Texel (n=45), Dorset (n=46), Chinese Merino (n=40), and BB group (n=149), B+ group (n=122), ++ group (n=36) from Small Tail Han, respectively. In Small Tail Han sheep, linkage analysis indicated that there was certain linkage disequilibrium between 100 bp allele of microsatellite BMS2508 and B allele of FecB gene (D' =0.408), and certain linkage disequilibrium between 110 bp and 114 bp alleles of microsatellite BMS2508 and + allele of FecB gene (D'=0.513).

Published
2009

30. [Advances on related genes with sexual precocity in mammals]

Author

Ming-Xing, Chu, Tao, Feng, Ran, DI, Bao-Yun, Zhang, and Ying-Jie, Zhang

Subjects
Receptors, Estrogen, Progesterone Reductase, GTP-Binding Protein alpha Subunits, Gs, Animals, Gene Expression Regulation, Developmental, Humans, Puberty, Precocious, Receptors, FSH, Sexual Maturation, Transforming Growth Factor alpha, Receptors, G-Protein-Coupled
Abstract

In mammals and humans, reproductive capacity is attained at puberty as the end-point of a complex series of developmental and neuroendocrine events that lead to true sexual maturity. As for humans, sexual precocity looks like a pathologic status. While for some animals, sexual precocity may be a valuable quantitative character. For some species, the character of sexual precocity was developed in the evolutionary process and stably transmitted to future generations. Sexual precocity is a complex character determined by polygenes. This review introduced the association between KiSS-1, GPR54, LHR, FSHR, CYP, ER, TGFa, IGF-, GNAS1, HSD3B2, SHBG, VDR genes and sexual precocity in mammals.

Published
2009

31. [Advances on progesterone receptor gene]

Author

Bao-Yun, Zhang, Ran, DI, Ming-Xing, Chu, Ping-Qing, Wang, and Lang, Lu

Subjects
Reproduction, Animals, Humans, Receptors, Progesterone, Polymorphism, Single Nucleotide
Abstract

The steroid hormone, progesterone, plays a key role in diverse events associated with female reproduction. In humans and other vertebrates, the biological activity of progesterone is mediated by modulation of the transcriptional activity of two progesterone receptors, PGR-A and PGR-B. This review introduced the structure, expression regulation and polymorphism of progesterone receptor gene. The relationship between progesterone receptor gene and reproductive function was also discussed in mammals.

Published
2008

32. [KISS-1/GPR54 genes and their role in reproduction]

Author

Tao, Feng, Ming-Xing, Chu, and Ying-Jie, Zhang

Subjects
Kisspeptins, Reproduction, Tumor Suppressor Proteins, Animals, Humans, Models, Biological, Receptors, G-Protein-Coupled, Receptors, Kisspeptin-1
Abstract

KISS-1 gene and its receptor gene GPR54 play key roles in the initiation of puberty onset. The peptide product of the KiSS-1 gene, Kisspeptins stimulate gonadotrophins release to initiate puberty through the expression of GPR54 gene in the brain. So the level of KISS-1 and GPR54 mRNA in hypothalamus was very high on the onset of puberty. The expression of KISS-1gene was regulated by steroid hormone in different nuclei within the forebrain to control the reproduction in puberty. Loss of function mutations of GPR54 gene could cause idiopathic hypogonadotropic hypogonadism (IHH) and gonadotrophin-dependant premature puberty. This review also introduced the structure, expression, homology comparison, polymorphism of KISS-1 and GPR54 genes and their interrelation with other regulators of reproduction.

Published
2008

33. Glucose sensor using a phospholipid polymer-based enzyme immobilization method

Author

Tamon Yagi, Kohji Mitsubayashi, Ming Xing Chu, Yasuhiko Iwasaki, Kazunari Akiyoshi, Hirokazu Saito, Hiroyuki Kudo, and Nobuyuki Morimoto

Subjects
Immobilized enzyme, Polymers, Phosphorylcholine, Biosensing Techniques, Methacrylate, Biochemistry, Analytical Chemistry, Enzyme catalysis, Glucose Oxidase, Glucose oxidase, Phospholipids, chemistry.chemical_classification, Reproducibility, Chromatography, biology, Molecular Structure, Chemistry, Reproducibility of Results, Polymer, Enzymes, Immobilized, Membrane, Glucose, Calibration, biology.protein, Methacrylates, Biosensor
Abstract

An electroenzymatic glucose sensor based on a simple enzyme immobilization technique was constructed and tested. The glucose sensor measures glucose concentrations as changes of oxygen concentrations induced by enzymatic reactions. The immobilizing procedure was developed with the purpose of producing wearable biosensors for clinical use. Two types of biocompatible polymers, 2-methacryloyloxyethyl phosphorylcholine (MPC) copolymerized with dodecyl methacrylate (PMD) and MPC copolymerized with 2-ethylhexyl methacrylate, were compared as a sensitive membrane of biosensors. The PMD enzyme membrane had a better response time. Linearity, reproducibility, effect of the concentrations of immobilized enzyme and drifts of sensor characteristics in long-term tests were also investigated. The linear characteristics were confirmed with glucose concentration from 0.01 to 2.00 mmol/l, with a coefficient of determination of 0.9999. The average output current for 1 mmol/l and the standard deviation were 0.992 and 0.0283 muA. Significant changes in the sensor's characteristics were not observed for 2 weeks when it was kept in a refrigerator at 4 degrees C. Because of the simple procedure, the enzyme immobilization method is not only useful for wearable devices but also other devices such as micro total analysis systems.

Published
2007

34. [Polymorphism of exon 10 of prolactin receptor gene and its relationship with prolificacy of Jining Grey goats]

Author

Li Fang, Gen-Xi Zhang, Ming-Xing Chu, Su-Cheng Ye, and Jin-Yu Wang

Subjects
Male, Genotype, Litter Size, Receptors, Prolactin, Molecular Sequence Data, Single-nucleotide polymorphism, Biology, Polymerase Chain Reaction, Polymorphism, Single Nucleotide, Angora goat, Exon, Gene Frequency, Cashmere goat, Animals, 3' Flanking Region, Gene, Polymorphism, Single-Stranded Conformational, Genetics, Polymorphism, Genetic, Base Sequence, Goats, General Medicine, Exons, Major gene, Molecular biology, Boer goat, Female
Abstract

Prolactin receptor (PRLR) gene was studied as a candidate gene for the prolificacy of Jining Grey goats. Five pairs of primers were designed to detect single nucleotide polymorphisms of exon 10 and part of 3'untranslated region (UTR) of PRLR gene in both high fecundity breed (Jining Grey goat) and low fecundity breeds (Liaoning Cashmere goat, Boer goat and Angora goat) by PCR-SSCP. The nucleotide sequence of exon 10 and part of 3'UTR of caprine PRLR gene was spliced in this study for the first time. The length of this sequence was 1,118 bp. This sequence shared 98.33%, 93.92%, 74.52% homology with the published mRNA of PRLR gene of sheep, cow and human separately, and shared 78.29% homology with the published partial genomic sequence of PRLR gene of the alpaca. Only the products amplified by primers P1, P2, P4 displayed polymorphisms. For primer P1, two genotypes (AA and AB) were detected in both Jining Grey goats and Liaoning Cashmere goats, two genotypes (AA and AC) were detected in Angora goats, and only genotype AA was detected in Boer goats. Sequencing revealed two mutations (186G-->A and 220T-->C) of PRLR gene in the genotype AB in comparison to the genotype AA. The former mutation resulted in an amino acid change of Asp-->Asn, and the latter mutation resulted in an amino acid change of Leu-->Pro. Only one mutation (140A-->G) was found in the genotype AC in comparison to the genotype AA, and this mutation did not cause any amino acid change. The difference of the least squares means (LSM) for litter size between AA and AB was non-significant (P>0.05) in Jining Grey goats. For primer P2, two genotypes (DD and DE) were detected in Jining Grey goats, Liaoning Cashmere goats and Boer goats, and only genotype DD was detected in Angora goats. Sequencing revealed two mutations (52G-->A and 122G-->A) of PRLR gene in the genotype DE in comparison to the genotype DD. The former mutation did not cause any amino acid change, and the latter mutation resulted in an amino acid change of Arg-->Gly. The difference of LSM for litter size between DD and DE was non-significant (P>0.05) in Jining Grey goats. For primer P4, two genotypes (FF and FG) were detected in Jining Grey goats, two genotypes (FF and GG) were detected in Liaoning Cashmere goats, only genotype FF was detected in Boer goats, and three genotypes (FF, FG and GG) were detected in Angora goats. Sequencing revealed one mutation (143A-->G) of PRLR gene in the genotype GG in comparison to the genotype FF, and this mutation resulted in an amino acid change of Met-->Val. The Jining Grey does with genotype FG had 0.76 (P< 0.05) kids more than those with genotype FF. These results preliminarily showed that the PRLR gene is either a major gene that influences the prolificacy of Jining Grey goats or a molecular marker in close linkage with such a gene.

Published
2007

35. [Estrogen receptor as a candidate gene for prolificacy of small tail Han sheep]

Author

Xiao-Dan, Bi, Ming-Xing, Chu, Hai-Guo, Jin, Li, Fang, and Su-Cheng, Ye

Subjects
Male, China, Base Sequence, Genotype, Litter Size, Exons, Sequence Analysis, DNA, Breeding, Polymerase Chain Reaction, Polymorphism, Single Nucleotide, Fertility, Gene Frequency, Receptors, Estrogen, Animals, Female, Alleles, Polymorphism, Single-Stranded Conformational, Sheep, Domestic
Abstract

Single nucleotide polymorphism in exon 1 of the estrogen receptor (ESR) gene was detected by PCR-SSCP in both high fecundity sheep breeds (Small Tail Han sheep, Hu sheep and German Mutton Merino sheep) and low fecundity sheep breeds (Dorset sheep,Suffolk sheep). Results indicated that there were three genotypes (AA, AB and BB) in all three high fecundity sheep breeds, but only two genotypes (AA, AB) in both low fecundity breeds. In Hu sheep,German Mutton Merino sheep, Small Tail Han sheep, Suffolk sheep and Dorset sheep,the frequency of allele A was 0.672, 0.786, 0.846, 0.857 and 0.867, respectively, and the frequency of allele B was 0.328, 0.214, 0.154, 0.143, and 0.133, respectively. Sequencing revealed a C--G mutation at 363 bp of exon 1 of ESR gene in the BB genotype in comparison to the AA genotype. The genotype distribution was significantly different between Small Tail Han sheep and Hu sheep (P0.01) and between Dorset sheep and Hu sheep (P0.05). There was no difference in genotype distribution between other sheep breeds. The Small Tail Han sheep ewes with genotypes AB or BB had 0.51 (P0.05) and 0.7 (P0.05) more lambs than those with genotype AA, respectively. These results showed that the estrogen receptor locus is either a major gene that influences the prolificacy in Small Tail Han sheep or in close linkage with such a gene. In view of our results, marker-assisted selection using ESR is warranted to increase litter size in sheep and will be of considerable economic value to mutton producers.

Published
2005

36. [Progress on prolactin receptor gene]

Author

Yu-Lian, Mu, Shao-Hua, Sun, and Ming-Xing, Chu

Abstract

This review introduced the structure of prolactin receptor,the developmental expression and function, action mechanism and molecular regulation, mapping of prolactin receptor gene and its relationship with reproductive traits. These revealed that prolactin receptor gene could be used as a candidate gene for reproductive traits.

Published
2005

37. [Study on relationships between seven microsatellite loci and somatic cell score in Beijing Holstein cows]

Author

Ming-Xing, Chu, Guo-Li, Zhou, Hai-Guo, Jin, Wan-Hai, Shi, Fu-Cun, Cao, Li, Fang, Su-Cheng, Ye, and Yan, Zhu

Subjects
China, Milk, Polymorphism, Genetic, Quantitative Trait, Heritable, Genotype, Animals, Cattle, Cell Count, Female, Chromosomes, Mammalian, Mastitis, Bovine, Microsatellite Repeats
Abstract

Genetic variation of seven microsatellite loci BM1818, BM1258, BM1443, BM1905, BM302, BM4505 and CYP21 which were closely linked to somatic cell score (SCS) was analyzed in 240 Beijing Holstein cows with nondenaturing polyacrylamide gel electrophoresis. Allele frequencies, heterozygosity, polymorphic information content, the effective number of alleles of seven microsatellite loci were calculated. Relationships between seven microsatellite loci and somatic cell score in Beijing Holstein cows were primarily analyzed by least squares linear model. Least squares means of SCS for BM1818 (284 bp/284 bp), BM1258 (106 bp/92 bp), BM1443 (166 bp/160 bp), BM1905 (187 bp/187 bp), BM302 (142 bp/140 bp), BM4505 (240 bp/236 bp) and CYP21 (215 bp/198 bp) were relatively lower,and their genotypes were the most favorable genotypes in respective locus for mastitis resistance. Least squares means of SCS for BM1818 (286 bp/286 bp), BM1258 (102 bp/102 bp), BM1443 (170 bp/160 bp), BM1905 (197 bp/195 bp), BM302 (154 bp/145 bp), BM4505 (240 bp/238 bp) and CYP21 (204 bp/192 bp) were relatively higher,and their genotypes were the most unfavorable genotypes in respective locus for mastitis resistance. The information found in the present study would be very important for improving mastitis resistance in dairy cattle by marker assisted selection.

Published
2005

38. [Study on BMP15 and GDF9 as candidate genes for prolificacy of Small Tail Han sheep]

Author

Ming-Xing, Chu, Lin-Hua, Sang, Jin-Yu, Wang, Li, Fang, and Su-Cheng, Ye

Subjects
Sheep, Gene Frequency, Genotype, Litter Size, Reproduction, Mutation, Animals, Growth Differentiation Factor 9, Intercellular Signaling Peptides and Proteins, Female, Polymerase Chain Reaction, Polymorphism, Restriction Fragment Length
Abstract

Bone morphogenetic protein 15 (BMP15) gene and growth differentiation factor 9 (GDF9) gene which control the fecundity of Belclare and Cambridge ewes were studied as candidate genes on the prolificacy of Small Tail Han sheep. Single nucleotide polymorphism of GDF9 gene and BMP15 gene was detected in both high fecundity sheep breeds (Small Tail Han sheep and Hu sheep) and low fecundity sheep breeds (Dorset sheep, Texel sheep and German Mutton Merino sheep) by PCR-RFLP. The results showed that the G8 mutation (C --T) of GDF9 gene and the B4 mutation (G --T) of BMP15 gene were not detected in five sheep breeds. There was the same B2 mutation (C --T) of BMP15 gene in Small Tail Han sheep as that in Belclare and Cambridge ewes. The same B2 mutation did not exist in other four sheep breeds. Concerning the B2 mutation of BMP15 gene, AA and AB genotypes were detected in Small Tail Han sheep, frequency of A allele was 0. 734, frequency of B allele was 0.266. The BMP15 B2 genotype distributions were high significantly different (P0.001) between Small Tail Han sheep and other four sheep breeds. The ewes with heterozygous mutant AB had 0.62 (P0.01) lambs more than those with wild homozygous type AA in Small Tail Han sheep. These results indicated that the B2 mutation of BMP15 gene had significant effect on the fecundity of Small Tail Han sheep and ruled out the possibility that the fecundity of Small Tail Han sheep was affected by the G8 mutation of GDF9 gene and the B4 mutation of BMP15 gene.

Published
2005

40. [Advances on inhibin genes]

Author

Yu, Xue, Ming-Xing, Chu, and Zhong-Xiao, Zhou

Subjects
Male, Polymorphism, Genetic, Litter Size, Reproduction, Chromosome Mapping, Prostatic Neoplasms, Primary Ovarian Insufficiency, Pancreatic Neoplasms, Gene Expression Regulation, Animals, Humans, Female, Inhibins, RNA, Messenger, Cloning, Molecular
Abstract

Inhibins are gonadal glycoprotein hormones belonging to the transforming growth factor-beta superfamily that act to suppress pituitary follicle-stimulating hormone synthesis and secretion. In this paper, we briefly introduced the cloning, structure, localization, polymorphism, expression, molecular regulation of inhibin-alpha(INHA), -betaA (INHBA) and -beta B (INHBB) subunit genes and their relationships with reproductive performance and cancer. The inhibin genes (INHA, INHBA and INHBB) had significant effect on litter size in sheep. The ovine INHA, INHBA and INHBB genes had been mapped to chromosomes 2q41--q43, 4q26 and 2q31--q33, respectively. The female mice carrying INHBB mutations suffered from distinct developmental and reproductive defects. The INHA gene was significantly associated with premature ovarian failure in women.

Published
2005

41. [Genetic relationships among seven sheep populations using four microsatellite markers]

Author

Ji-Zhen, Wang, Ming-Xing, Chu, Ai-Guo, Wang, Ning, Li, Jin-Lian, Fu, Fang, Xie, and Guo-Hong, Chen

Subjects
Male, China, Heterozygote, Polymorphism, Genetic, Sheep, Genetic Variation, Breeding, Polymerase Chain Reaction, Gene Frequency, Animals, Female, Alleles, Phylogeny, Microsatellite Repeats
Abstract

The genetic polymorphisms of four microsatellite loci BM143, OarHH35, OarAE101, and BMS2508 were analyzed in 286 sheep of seven sheep populations (Small Tail Han sheep, Hu sheep, Ujumqin sheep, Suffolk sheep, Dorset sheep, Charolais sheep, F1 of Dorset male x Small Tail Han female sheep). The numbers of alleles for BM143, OarHH35, OarAE101, and BMS2508 are 9, 11, 14 and 9 in seven sheep populations, respectively. The polymorphism information content/number of effective alleles/ heterozygosity of BM143, OarHH35, OarAE101 and BMS2508 were 0.7073/3.7231/0.7314, 0.8267/6.4399/0.8447, 0.5743/2.5178/0.6028, 0.6172/3.0712/0.6744 in 286 sheep, respectively. The results revealed the greatest genetic variation at OarHH35 locus and the lowest at OarAE101, the greatest genetic variation in Small Tail Han sheep and the lowest in Hu sheep among seven sheep populations. In the unweighted pair group method with arithmetic mean (UPGMA) dendrograms based on Nei's D(A) distance and Nei's D(S) standard genetic distance, the Chinese native breeds (Small Tail Han sheep, Ujumqin sheep, Hu sheep) were grouped together, then with Charolais sheep. The F1 crossbred sheep, and the two British native sheep (Suffolk sheep, Dorset sheep) also clustered together. Microsatellite genotyping in sheep provided a useful tool for examining the genetic relationships among breeds (populations).

Published
2005

42. [Genetic variation of A-FABP microsatellites in eleven pig breeds]

Author

Zhen, Li, Ming-Xing, Chu, Hong-He, Cao, Hong-Bin, Li, Yue-Hui, Ma, You-Min, Zheng, and Zhong-Xiao, Zhou

Subjects
China, Heterozygote, Polymorphism, Genetic, Gene Frequency, Swine, Animals, Breeding, Fatty Acid-Binding Proteins, Alleles, Introns, Microsatellite Repeats
Abstract

The genetic variations of microsatellites in intron 2 of the porcine adipocyte fatty acid-binding protein (A-FABP) genes were investigated in 420 pigs including Wuzhishan pig, Yimeng black pig, Hanjiang black pig, Laiwu pig, Beijing black pig, Min pig, Chenghua pig, Neijiang pig, Erhualian pig, Bama xiang pig and Large White pig. The results suggested as follows: (i)PIC of the Wuzhishan pig breed is the highest (0.7904) and 11 alleles were detected. Compared with Large White pig,Chinese pig breeds showed a great polymorphism of A-FABP microsatellites except Beijing black pig in which only 2 alleles were detected. (ii) Only Min pig, Bama xiang pig, Beijing black pig and Large White pig were in Hardy-Weinberg equilibrium. (iii) The analysis of genetic differentiation showed that the average value of the A-FABP gene differentiation of 10 Chinese pigs is about 40.83%.

Published
2005

43. [Advances on melatonin receptor gene]

Author

Cong-Liang, Ji, Ming-Xing, Chu, and Guo-Hong, Chen

Abstract

Melatonin exerts its biological effects through pharmacological specific, high affinity G protein-coupled receptors. This review introduced the structure, function, and regulation of melatonin receptor,the cloning and structure, developmental expression, mapping and polymorphism of melatonin receptor gene. The relationship between melatonin receptor gene and reproductive seasonality was also discussed.

Published
2005

45. [Molecular biology of the retinol-binding proteins and their genes]

Author

Xiao-Hong, Guo, Ming-Xing, Chu, and Zhong-Xiao, Zhou

Subjects
Retinol-Binding Proteins, Gene Expression Regulation, Liver, Uterus, Animals, Chromosome Mapping, Humans, Female, Retinol-Binding Proteins, Cellular, RNA, Messenger, Breeding, Kidney, Vitamin A
Abstract

Retinol-binding proteins (RBPs) are a kind of circulating carrier proteins for serum and cellular retinol and retinol acid, which are lipid-soluble vitamins, and are members of hydrophobic binding protein family. Serum RBPs were synthesized primarily in liver, then was released into blood streams, and then to various tissues. Under the interaction with substances such as retinol, pre-albumin and the receptors of cellular surface, they play important roles in storage, metabolism of VitA and transport of VitA to the target cells. Cellular RBPs play the similar function as serum RBPs in intracell. This review introduces action mechanism, tissue localization and developmental expression of retinol-binding proteins. This review also introduces the structure, chromosome mapping and their relationships with reproductive performance of retinol-binding protein genes.

Published
2005

46. [Research progress on myogenin gene]

Author

Yuan-Qing, He, Ming-Xing, Chu, and Jin-Yu, Wang

Subjects
Gene Expression Regulation, Genes, Regulator, Animals, Humans, Sequence Homology, Myogenin, Muscle Development, Muscle, Skeletal, Chromosomes, Mammalian, Polymerase Chain Reaction, Polymorphism, Restriction Fragment Length, Polymorphism, Single-Stranded Conformational
Abstract

In this paper we briefly introduced the location, structure, polymorphisms of myogenin gene, and discussed the relationships of myogenin gene with economic traits.

Published
2005

47. [Progress on the sheep genome project]

Author

Xiao-Hong, Guo, Ming-Xing, Chu, and Zhong-Xiao, Zhou

Subjects
Genetic Markers, Sheep, Quantitative Trait Loci, Body Composition, Animals, Chromosome Mapping, Chromosomes, Mammalian
Abstract

During the last few years,advances in livestock genome projects have been remarkable. Species-specific genetic maps exist for pig, chicken, cattle, sheep, horse,and deer with marker intervals of 5 to 20 cM. These maps have been essential for the identification of genes and genetic markers associated with importantly economic traits in livestock. In this paper, advances of gene map, comparative map, the genes for importantly economic traits and quantitative trait loci (QTL) mapping were briefly introduced in sheep.

Published
2005

48. [PCR-SSCP analysis on growth differentiation factor 9 gene in sheep]

Author

Bi-Xia, Li, Ming-Xing, Chu, and Jin-Yu, Wang

Subjects
Sheep, Gene Frequency, Genotype, DNA Mutational Analysis, Mutation, Animals, Growth Differentiation Factor 9, Intercellular Signaling Peptides and Proteins, DNA, Polymerase Chain Reaction, Polymorphism, Single Nucleotide, Polymorphism, Single-Stranded Conformational
Abstract

Growth differentiation factor 9 (GDF9) is a growth factor secreted by oocytes in growing ovarian follicles, which is essential for growth and differentiation of early ovarian follicles. The polymorphism of GDF9 gene in Small Tail Han sheep, Hu sheep, Dorset sheep and Suffolk sheep was analyzed by PCR-SSCP. The results indicated that there were three genotypes (AA, AB and BB) detected by primer 1. AA genotype was detected in four sheep breeds. AB genotype was detected in Hu sheep, Dorset sheep and Suffolk sheep. BB genotype was only detected in Suffolk sheep. Frequency of A allele was obviously higher than frequency of B allele in four sheep breeds. There were two genotypes (AA and AB) detected by primer 2. AA genotype was detected in four sheep breeds. AB genotype was detected in Hu sheep, Dorset sheep and Suffolk sheep. BB genotype was not detected in four sheep breeds. Frequency of AA genotype was the highest, and frequency of A allele was obviously higher than frequency of B allele in four sheep breeds. The polymorphic fragments amplified by primer 1 were cloned and sequenced. The sequencing results showed that there was one single nucleotide mutation: A--G at cDNA 152 of GDF9 gene in sheep, and this mutation resulted in an amino acid change: asparagine--aspartic acid.

Published
2003

49. [Genetic polymorphisms of five microsatellite loci in Small Tail Han sheep]

Author

Ming-Xing, Chu, Ji-Zhen, Wang, Ai-Guo, Wang, Ning, Li, and Jin-Lian, Fu

Subjects
DNA, Complementary, Polymorphism, Genetic, Sheep, Base Sequence, Gene Frequency, Molecular Sequence Data, Animals, Female, Microsatellite Repeats
Abstract

Small Tail Han sheep is an excellent local sheep breed in China. Small Tail Han sheep had significant characteristics of high prolificacy. The lambing percentage averaged 260 percent in Small Tail Han sheep. The polymorphisms of 5 microsatellite loci OarAE101, BM1329, BMS2508, TGLA54 and TGLA68 which were closely linked to the fecundity genes FecB and FecXI in sheep were detected in 244 ewes of Small Tail Han sheep. The PCR amplified products of microsatellites were detected by non-denatured (natural) polyacry lamide gel electrophoresis. Allele frequency, polymorphism information content, gene homogeneity and heterozygosity for 5 microsatellite loci were calculated. The number of alleles for BM1329, OarAE101, TGLA54, TGLA68 and BMS2508 were 6, 9, 5, 2 and 6 in Small Tail Han sheep, respectively. The range of allele sizes for BM1329, OarAE101, TGLA54, TGLA68 and BMS2508 were 160 bp to 180 bp, 97 bp to 135 bp, 116 bp to 136 bp, 98 bp to 100 bp, and 93 bp to 115 bp, respectively. The alleles of the greatest frequency for BM1329, OarAE101, TGLA54 and BMS2508 were 164 bp, 97 bp, 134 bp and 99 bp, respectively. Polymorphism information content/gene homogeneity/heterozygosity for BM1329, OarAE101, TGLA54, TGLA68 and BMS2508 were 0.4481/0.4840/0.5160, 0.3516/0.6375/0.3625, 0.2528/0.7326/0.2674, 0.3733/0.5034/0.4966 and 0.5809/0.3581/0.6419 in Small Tail Han sheep, respectively. The results revealed the greatest genetic variation in BMS2508 and the lowest in TGLA54. These results could provide, basic molecular data for the research on the germplasm characteristics of Small Tail Han sheep.

Published
2002

50. [Cloning and sequencing of four microsatellite loci in Small Tail Han Sheep]

Author

Ming-Xing, Chu, Ji-Zhen, Wang, Ai-Guo, Wang, Ning, Li, and Jin-Lian, Fu

Subjects
Male, Sheep, Base Sequence, Sequence Homology, Nucleic Acid, Molecular Sequence Data, Animals, Female, DNA, Sequence Analysis, DNA, Cloning, Molecular, Sequence Alignment, Microsatellite Repeats, Pedigree
Abstract

Small Tail Han sheep is an excellent local sheep breed in China. Small Tail Han sheep has significant characteristics of high prolificacy. The lambing percentage averaged 260 percent in Small Tail Han sheep. The genetic detection of 4 microsatellite loci OarAE101, OarHH35, BM143 and BMS2508 which were closely linked to the fecundity gene FecB in Booroola sheep was conducted in 159 sheep in Small Tail Han sheep, Dorset sheep, F1 hybzids(Dorset x Small Tail Han sheep). The results confirmed the genetic characteristics of codominance of microsatellite DNA. The PCR amplified products of microsatellites were detected by non-denatured (natural) polyacrylamide gel electrophoresis. The sequences of PCR amplification fragment of 6 clones of 4 microsatellite loci in Small Tail Han sheep were accepted by GenBank of National Center for Biotechnology Information, National Institutes of Health in USA, the GenBank accession numbers were AF394445, AF394446, AF394447, AF394448, AF394449, AF394450, respectively. The sequence homogeneity between OarAE101 in Small Tail Han sheep in this study and the ovine OarAE101 in GenBank was 98 percent. The sequence homogeneity between OarHH35 in Small Tail Han sheep in this study and the ovine OarHH35 in GenBank was 99 percent. The sequence homogeneity between BM143 in Small Tail Han sheep in this study and the bovine BM143 in GenBank was 95 percent. The sequence homogeneity between BMS2508 in Small Tail Han sheep in this study and the bovine BMS2508 in GenBank was 95 percent. OarAE101, OarHH35, BM143 and BMS2508 in Small Tail Han sheep were all perfect microsatellites. These results could provide molecular basic data for the research on the germplasm characteristics of Small Tail Han sheep.

Published
2002

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