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Sex Ratio Determination by Quantitative Real Time PCR using Amelogenin Gene in Porcine Sperm
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  • Sex Ratio Determination by Quantitative Real Time PCR using Amelogenin Gene in Porcine Sperm
  • Sex Ratio Determination by Quantitative Real Time PCR using Amelogenin Gene in Porcine Sperm
저자명
Hwang. You-Jin,Bae. Mun-Sook,Yang. Jae-Hun,Kim. Bo-Kyoung,Kim. Sang-Ok,Lee. Eun-Soo,Choi. Sun-Gyu,Kwon. Ye-Ri,Seo. Min-Hae,Park.
간행물명
韓國受精卵移植學會誌
권/호정보
2009년|24권 3호|pp.225-230 (6 pages)
발행정보
한국수정란이식학회
파일정보
정기간행물|ENG|
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이 논문은 한국과학기술정보연구원과 논문 연계를 통해 무료로 제공되는 원문입니다.
서지반출

기타언어초록

Sex-sorting of sperm is an assisted reproductive technology (ART) used by the livestock industry for the mass production of animals of a desired sex. The standard method for sorting sperm is the detection of DNA content differences between X and Y chromosome-bearing sperm by flow cytometry. However, this method has variable efficiency and therefore requires verification by a second method. We have developed a sex determination method based on quantitative real-time polymerase chain reaction (qPCR) of the porcine amelogenin (AMEL) gene. The AMEL gene is present on both the X and the Y chromosome, but the length and sequence of its noncoding regions differ between the X and Y chromosomes. By measuring the threshold cycle (Ct) of qPCR, we were able to calculate the relative frequency of X chromosome. Two sets of AMEL primers were used in these studies. One set (AME) targeted AMEL gene sequences present in both X and Y chromosome, but produced PCR products of different lengths for each chromosome. The other set (AXR) bound to AMEL gene sequences present on the X chromosome but absent esholthe Y-chromosome. Relative product levels were calculated by normalizing the AXR fluorescence to the AME fluorescence. The AMEL method accurately predicted the sex ratios of boar sperm, demonstrating that it has potential value as a sex determination method.