Your search keyword '"Zhang, Xiangzhe"' showing total 4 results

1. An Efficient Genotyping Method in Chicken Based on Genome Reducing and Sequencing.

Author

Liao, Rongrong, Wang, Zhen, Chen, Qiang, Tu, Yingying, Chen, Zhenliang, Wang, Qishan, Yang, Changsuo, Zhang, Xiangzhe, and Pan, Yuchun

Subjects

SINGLE nucleotide polymorphisms, GENOTYPES, NUCLEOTIDE sequencing, CHROMOSOMES, CHICKENS

Abstract

Single nucleotide polymorphisms (SNPs) are essential for identifying the genetic mechanisms of complex traits. In the present study, we applied genotyping by genome reducing and sequencing (GGRS) method to construct a 252-plex sequencing library for SNP discovery and genotyping in chicken. The library was successfully sequenced on an Illumina HiSeq 2500 sequencer with a paired-end pattern; approximately 400 million raw reads were generated, and an average of approximately 1.4 million good reads per sample were generated. A total of 91,767 SNPs were identified after strict filtering, and all of the 252 samples and all of the chromosomes were well represented. Compared with the Illumina 60K chicken SNP chip data, approximately 34,131 more SNPs were identified using GGRS, and a higher SNP density was found using GGRS, which could be beneficial for downstream analysis. Using the GGRS method, more than 3528 samples can be sequenced simultaneously, and the cost is reduced to $18 per sample. To the best of our knowledge, this study describes the first report of such highly multiplexed sequencing in chicken, indicating potential applications for genome-wide association and genomic selection in chicken. [ABSTRACT FROM AUTHOR]

Published

2015

2. Transgenic Mice Expressing Yeast CUP1 Exhibit Increased Copper Utilization from Feeds.

Author

Xie, Xiaoxian, Ma, Yufang, Chen, Zhenliang, Liao, Rongrong, Zhang, Xiangzhe, Wang, Qishan, and Pan, Yuchun

Subjects

YEAST fungi genetics, GENE expression, COPPER, TRANSGENIC mice, GENETIC regulation, MICRONUTRIENTS, PLASMID genetics

Abstract

Copper is required for structural and catalytic properties of a variety of enzymes participating in many vital biological processes for growth and development. Feeds provide most of the copper as an essential micronutrient consumed by animals, but inorganic copper could not be utilized effectively. In the present study, we aimed to develop transgenic mouse models to test if copper utilization will be increased by providing the animals with an exogenous gene for generation of copper chelatin in saliva. Considering that the S. cerevisiae CUP1 gene encodes a Cys-rich protein that can bind copper as specifically as copper chelatin in yeast, we therefore constructed a transgene plasmid containing the CUP1 gene regulated for specific expression in the salivary glands by a promoter of gene coding pig parotid secretory protein. Transgenic CUP1 was highly expressed in the parotid and submandibular salivary glands and secreted in saliva as a 9-kDa copper-chelating protein. Expression of salivary copper-chelating proteins reduced fecal copper contents by 21.61% and increased body-weight by 12.97%, suggesting that chelating proteins improve the utilization and absorbed efficacy of copper. No negative effects on the health of the transgenic mice were found by blood biochemistry and histology analysis. These results demonstrate that the introduction of the salivary CUP1 transgene into animals offers a possible approach to increase the utilization efficiency of copper and decrease the fecal copper contents. [ABSTRACT FROM AUTHOR]

Published

2014

3. A New Genotype Imputation Method with Tolerance to High Missing Rate and Rare Variants.

Author

Yang, Yumei, Wang, Qishan, Chen, Qiang, Liao, Rongrong, Zhang, Xiangzhe, Yang, Hongjie, Zheng, Youmin, Zhang, Zhiwu, and Pan, Yuchun

Subjects

INFORMATION theory, MOLECULAR genetics, SEQUENCE analysis, POPULATION genetics, COMPUTATIONAL biology, ANIMAL genetics, ALGORITHMS

Abstract

We report a novel algorithm, iBLUP, to impute missing genotypes by simultaneously and comprehensively using identity by descent and linkage disequilibrium information. The simulation studies showed that the algorithm exhibited drastically tolerance to high missing rate, especially for rare variants than other common imputation methods, e.g. BEAGLE and fastPHASE. At a missing rate of 70%, the accuracy of BEAGLE and fastPHASE dropped to 0.82 and 0.74 respectively while iBLUP retained an accuracy of 0.95. For minor allele, the accuracy of BEAGLE and fastPHASE decreased to −0.1 and 0.03, while iBLUP still had an accuracy of 0.61.We implemented the algorithm in a publicly available software package also named iBLUP. The application of iBLUP for processing real sequencing data in an outbred pig population was demonstrated. [ABSTRACT FROM AUTHOR]

Published

2014

4. Genotyping by Genome Reducing and Sequencing for Outbred Animals.

Author

Chen, Qiang, Ma, Yufang, Yang, Yumei, Chen, Zhenliang, Liao, Rongrong, Xie, Xiaoxian, Wang, Zhen, He, Pengfei, Tu, Yingying, Zhang, Xiangzhe, Yang, Changsuo, Yang, Hongjie, Yu, Fuqing, Zheng, Youmin, Zhang, Zhiwu, Wang, Qishan, and Pan, Yuchun

Subjects

NUCLEOTIDE sequence, AGRICULTURAL biotechnology, COMPUTATIONAL biology, POPULATION genetics, GENETIC polymorphisms, POPULATION biology, ANIMAL models in research

Abstract

Next-generation sequencing (NGS) approaches are widely used in genome-wide genetic marker discovery and genotyping. However, current NGS approaches are not easy to apply to general outbred populations (human and some major farm animals) for SNP identification because of the high level of heterogeneity and phase ambiguity in the haplotype. Here, we reported a new method for SNP genotyping, called genotyping by genome reducing and sequencing (GGRS) to genotype outbred species. Through an improved procedure for library preparation and a marker discovery and genotyping pipeline, the GGRS approach can genotype outbred species cost-effectively and high-reproducibly. We also evaluated the efficiency and accuracy of our approach for high-density SNP discovery and genotyping in a large genome pig species (2.8 Gb), for which more than 70,000 single nucleotide polymorphisms (SNPs) can be identified for an expenditure of only $80 (USD)/sample. [ABSTRACT FROM AUTHOR]

Published

2013