Journal of Preventive Medicine and Public Health

The Korean Society for Preventive Medicine (대한예방의학회)
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Assessment of DNA Viability in Long term-Stored Buffy Coat Species for the Korean Multicenter Cancer Cohort

한국인 다기관 암 코호트 시료의 DNA 생활성도 평가

  • Yang, Mi-Hi (Department of Preventive Medicine, Seoul National University College of Medicine) ;
  • Yoo, Ji-Hyun (Department of Preventive Medicine, Seoul National University College of Medicine) ;
  • Kim, Cheong-Sik (Department of Preventive Medicine, Seoul National University College of Medicine) ;
  • Shin, Ae-Sun (Department of Preventive Medicine, Seoul National University College of Medicine) ;
  • Kang, Dae-Hee (Department of Preventive Medicine, Seoul National University College of Medicine) ;
  • Chang, Soung-Hoon (Department of Preventive Medicine, Konkuk University College of Medicine) ;
  • Park, Sue-Kyung (Department of Preventive Medicine, Konkuk University College of Medicine) ;
  • Shin, Hai-Rim (Division of Cancer Control & Epidemiology, National Cancer Center) ;
  • Yoo, Keun-Young (Department of Preventive Medicine, Seoul National University College of Medicine)
  • 양미희 (서울대학교 의과대학 예방의학교실) ;
  • 유지현 (서울대학교 의과대학 예방의학교실) ;
  • 김청식 (서울대학교 의과대학 예방의학교실) ;
  • 신애선 (서울대학교 의과대학 예방의학교실) ;
  • 강대희 (서울대학교 의과대학 예방의학교실) ;
  • 장성훈 (건국대학교 의과대학 예방의학교실) ;
  • 박수경 (건국대학교 의과대학 예방의학교실) ;
  • 신해림 (국립암센터 암역학관리연구부) ;
  • 유근영 (서울대학교 의과대학 예방의학교실)
  • Published : 2003.12.01
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Abstract

Objectives : Peripheral blood-buffy coat fractions (N=14,956) have been stored at $-70^{\circ}C$ in the headquarter of the Korean Multicenter Cancer Cohort (KMCC), since 1993. To study the future molecular etiology of cancers using specimens of the cohort, properly stored specimens are necessary, Therefore, the DNA-viability of the bully coat samples was investigated. Methods : Buffy coat fraction samples were randomly selected from various collection areas and years (N=100). The DNA viability was evaluate from the UV-absorbent ratios at 260/280nm and the PCH for $\beta$-globin was performed with genomic DNA isolated from the buffy coat. Results : PCR products were obtained from 85 and 98% of the C and H area-samples, respectively, using 50 or $100{\mu}l$ of the buffy coat. There were significant differences in the yields of the PCR-amplifications from the C and H areas (p<0.05), which was due to differences in the homogenization of the buffy coat fractions available as aliquots. The PCR-products were obtained from all of the samples (N=7) stored at the C area-local confer, but the other aliquots stored at the headquarter were not PCR-amplified, Therefore, the PCR products in almost all the samples, even including the DNA-degraded samples, were obtained. In addition, an improvement in the DNA isolation, i,e. approx. 1.6 fold, was found after using extra RBC lysis buffer. Conclusions : PCR products for $\beta$-globin were obtained from nearly all of the samples. The regional differences in the PCR amplifications were thought to have originated from the different sample-preparation and homogenization performance. Therefore, the long term-stored buffy coat species at the KMCC can be used for future molecular studies.

Keywords

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