The Journal of the Korean Society for Microbiology (대한미생물학회지)

The Korea Society for Microbiology (대한미생물학회)
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Methods for Coating the Killed Whole Cell Antigens of Salmonella typhi in Enzyme-linked Immunosorbent Assay

효소면역측정법을 위한 장티푸스 균체항원의 부착방법

  • Kim, Youn-Won (Department of Microbiology, Cancer Research Institute, College of Medicine, Seoul National University) ;
  • Hwang, Eung-Soo (Department of Microbiology, Cancer Research Institute, College of Medicine, Seoul National University) ;
  • Kook, Yoon-Hoh (Department of Microbiology, Cancer Research Institute, College of Medicine, Seoul National University) ;
  • Choi, Kang-Won (Department of Internal Medicine, College of Medicine, Seoul National University) ;
  • Kim, Ik-Sang (Department of Microbiology, Cancer Research Institute, College of Medicine, Seoul National University) ;
  • Cha, Chang-Yong (Department of Microbiology, Cancer Research Institute, College of Medicine, Seoul National University) ;
  • Lee, Seung-Hoon (Department of Microbiology, Cancer Research Institute, College of Medicine, Seoul National University)
  • 김윤원 (서울대학교 의과대학 미생물학교실.암연구소) ;
  • 황응수 (서울대학교 의과대학 미생물학교실.암연구소) ;
  • 국윤호 (서울대학교 의과대학 미생물학교실.암연구소) ;
  • 최강원 (서울대학교 의과대학 내과학교실) ;
  • 김익상 (서울대학교 의과대학 미생물학교실.암연구소) ;
  • 차창용 (서울대학교 의과대학 미생물학교실.암연구소) ;
  • 이승훈 (서울대학교 의과대학 미생물학교실.암연구소)
  • Published : 1985.12.31
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Abstract

The advantages of enzyme-linked immunosorbent assay(ELISA) are its senstivity and simplicity in detecting IgG, IgM and IgA antibody. To apply ELISA to diagnosis of typhoid fever, antigen such as lipopolysaccharide of Salmonella typhi or killed whole cell must be coated on solid phase. It is easy to coat lipopolysaccharide on ELISA plate but troublesome to purify it. As it is easy to obtain the killed whole cells, the development of the appropriate method by which those antigens of S. typhi are optimally coated on solid phase is needed. To establish the appropriate method, carbonate buffer, methanol or poly-L-lysine was applied as binding substance on polystyrene or polyvinylchloride plate as solid phase when the killed whole cell antigens of S. typhi varided as follows: $10^6$, $10^7$, $10^8$ and $10^9\;cell/ml$. The criteria of the optimal method were determined as follows: 1. The optical density of positive sera is above 1.0(0.6 in IgM) at 1:10 serum dilution and is 0.3(0.2 in IgM) higher than that of negative sera: 2. The O.D. of sera is flat or lowering according to serum dilution: 3. It must be that the O.D. of negative sera is lower than 0.2 at the point of serum dilution where the O.D. of positive sera is higher than 1.0(0.5 in IgM). The results obtained were summarized as follows: 1. The methods which fitted the above criteria were to use poly-L-lysine as binding substance, polyvinylchloride plate as solid phase and $10^7\;cell/ml$ as antigen concentration of S. typhi(poly-L-lysine/polyvinylchloride/$10^7$) and poly-L-lysine/polyvinylchloride/$10^8$ in detecting IgG antibody, methanol/polystyrene/$10^9$, poly-L-lysine/polyvinylchloride/$10^8$ and poly-L-lysine/polyvinylchloride/$10^9$ in IgM and carbonate buffer/polystyrene/$10^8$, carbonate buffer/polystyrene/$10^9$, methanol/polystyrene/$10^8$, methanol/polyvinylchloride/$10^8$, methanol/polyvinylchloride/$10^9$, poly-L-lysine/polyvinylchloride/$10^8$ and poly-L-lysine/polyvinylchloride/$10^9$ in IgA. 2. The coaling method using poly-L-lysine, polyvinylchloride plate and $10^8\;cell/ml$ was best to assay IgG, IgM and IgA antibody all in one. By this method, to assay the each immunoglobulin calss with an appropriate fixed serum dilution, 1:320 dilution was best.

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