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KR980700433A - 디엔에이(dna) 시퀀싱 및 디엔에이(dna) 동정을 위한 방법 및 장치(methods and apparatus for dna sequencing and dna identification) - Google Patents

디엔에이(dna) 시퀀싱 및 디엔에이(dna) 동정을 위한 방법 및 장치(methods and apparatus for dna sequencing and dna identification)

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KR980700433A
KR980700433A KR1019970703847A KR19970703847A KR980700433A KR 980700433 A KR980700433 A KR 980700433A KR 1019970703847 A KR1019970703847 A KR 1019970703847A KR 19970703847 A KR19970703847 A KR 19970703847A KR 980700433 A KR980700433 A KR 980700433A
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nucleic acid
probes
probe
acid segments
hybridization
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라도제 티. 드르마낙
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그루버 루이스
하이세크, 인코포레이티드
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Abstract

본 발명은 다중 샘플의 다중 프로브 분석을 분리시키는 세분화된 필터를 채용하여 DNA 동정과 DNA 시퀀싱 용도로 사용될 수 있는, 하이브리디제이션에 의한 시퀀싱(SBH)방법 및 장치에 관한 것이다. 분할된 필터들은 제조되었다. 분할된 필터부에 샘플이 첨부되어, 각각의 색터가 하이브리디제이션 스코어링용으로 다중화된 프로브 또는 단일 프로브로 프로브된다. 하이브리디제에션 데이타는 프로브 완결성, SBH에 의한 부분 시퀀싱 또는 SBH에 의한 완전한 시퀀싱에 대해 분석된다.

Description

디엔에이(DNA) 시퀀싱 및 디엔에이(DNA) 동정을 위한 방법 및 장치(METHODS AND APPARATUS FOR DNA SEQUENCING AND DNA IDENTIFICATION)
본 내용은 요부공개 건이므로 전문내용을 수록하지 않았음

Claims (34)

  1. 기질의 제 1 섹터 상에 첫 번째 복수개의 핵산 세그먼트를 어레이시키고; 기질의 제 2 섹터 상에 두 번째 복수개의 핵산 세그먼트를 배치한 다음; 완전히 상보적인 것과 단일 염기 미스맷치를 구별할 수 있는 조건 하에서, 상기 제 1 섹터 중의 제 1 하이브리디제이션 프로브 (여기서 상기 제 1 하이브리디제이션 프로브는 상기 첫번째 복수개의 핵산 세그먼트 중 어느 하나 보다 짧음)에 첫 번째 복수개의 핵산 세그먼트를 노출시키고; 완전히 상보적인 것과 단일 염기 미스맷치를 구별할 수 있는 조건 하에서, 상기 제 2 섹터 중의 제 2 하이브리디제이션 프로브 (여기서 상기 제 2 하이브리디제이션 프로브는 상기 두번째 복수개의 핵산 세그먼트 중 어느 하나 보다 짧고 상기 첫 번째 복수개의 핵산 세그먼트와 상이함)를 인큐베이팅한 다음; 하이브리디제이션 프로브가 핵산 세그먼트에 하이브리디제이션 되었는지를 검색하여; 그 결과를 분석하는 단계로 이루어지는, 하이브리디제이션에 의한 핵산 분석 방법.
  2. 제 1항에 있어서, 상기 두 번째 복수개의 핵산 세그먼트의 배치 단계에 앞서, 핵산 이동을 막는 장벽을 도입하는 단계를 추가로 포함하는 방법.
  3. 제 1항에 있어서, 상기 첫 번째 핵산 세그먼트의 어레이 단계와 상기 두 번째 복수개의 핵산 세그먼트이 배치 단계 후, 상기 인큐베이션 단계 전에, 핵산 이동을 막는 장벽을 도입하는 단계를 추가로 포함하는 방법.
  4. 제 3항에 있어서, 상기 도입 단계가 물리적 장벽을 상기 기질에 대해 압착하는 단계인 방법.
  5. 제 2항에 있어서, 상기 도입 단계가 상기 지지체에 대해 수직인 방향-스위칭 전기장을 인가함으로써 섹터들 간의 프로브의 혼합을 방지하는 단계인 방법.
  6. 제 3항에 있어서, 상기 도입 단계가 상기 지지체에 대해 수직인 방향-스위칭 전기장을 인가함으로써 섹터들 간의 프로브의 혼합을 방지하는 단계인 방법.
  7. 제 1항에 있어서, 상기 어레이 단계가 핀 어레이 수단에 의해 핵산 샘플을 스포팅하는 단계로 이루어진 방법.
  8. 제 1항에 있어서, 상기 어레이 단계가 튜브 어레이에 의해 핵산 샘플을 배치하는 단계로 이루어진 방법.
  9. 제 1항에 있어서, 상기 어레이 단계가 핵산 샘플을 제트 프린팅하는 단계로 이루어진 방법.
  10. 제 1항에 있어서, 상기 노출 단계가 복수개의 인접하는 하이브리다이징 프로브들을 적용하는 단계로 이루어진 방법.
  11. 제 1항에 있어서, 상기 인큐베이팅 단계가 복수개의 인접하는 하이브리다이징 프로브들을 적용하는 단계로 이루어진 방법.
  12. 제 10항에 있어서, 2개 이상의 상기 복수개의 인접하는 하이브리다이징 프로브들을 라이게이팅시키는 단계를 출가로 포함하는 방법.
  13. 제 11항에 있어서, 2개 이상의 상기 복수개의 인접하는 하이브리다이징 프로브들을 라이게이팅시키는 단계를 출가로 포함하는 방법.
  14. 제 1항에 있어서, 상기 노출 단계가 중복되는 핵산 서열을 갖는 복수개의 경쟁적인 하이브리다이징 프로브들을 적용하는 단계로 이루어진 방법.
  15. 제 1항에 있어서, 상기 인큐베이선 단계가 중복되는 핵산 서열을 갖는 복수개의 경쟁적인 하이브리다이징 프로브들을 적용하는 단계로 이루어진 방법.
  16. 제 1항에 있어서, 2개 이상의 상기 첫 번째 복수개의 핵산 세그먼트들을 혼합물로서 배치하는 방법.
  17. 제 1항에 있어서, 2개 이상의 상기 두 번째의 복수개의 핵산 세그먼트들을 혼합물로서 배치하는 방법.
  18. 제 1항에 있어서, Hga I형 제한 효소를 이용한 절단과 그 결과 얻어진 제한 효소 절단된 단편들을 앵커를 이용하여 라이게이션시킴으로써 샘플을 제조하는 단계를 추가로 포함하는 방법.
  19. 제 1항에 있어서, 주어진 길이의 보편적인 프로브 세트로부터 프로브들을 선별하는 단계를 추가로 포함하는 방법.
  20. 제 1항에 있어서, 주어진 길이의 불완전한 프로브 세트로부터 프로브들을 선별하는 단계를 추가로 포함하는 방법.
  21. 제 1항에 있어서, 데옥시리보뉴클레오티드 프로브들을 선별하는 단계를 추가로 포함하는 방법.
  22. 제 1항에 있어서, 리보뉴클레오티드 프로브들을 선별하는 단계를 추가로 포함하는 방법.
  23. 제 1항에 있어서, 염기 동족체를 함유하는 프로브들과 단백질 핵산 프로브 그룹으로부터 핵산 동족체를 선별하는 단계를 추가로 포함하는 방법.
  24. 제 1항에 있어서, 프로브들을 다중 표지시키는 단계를 추가로 포함하는 방법.
  25. 제 1항에 있어서, 하이브리다이즈되지 않은 프로브 상의 표지를 분해시키는 단계를 추가로 포함하는 방법.
  26. 제 19항에 있어서, 상기 노출 단계 또는 상기 인큐베이팅 단계가 6, 7 8, 9 또는 10 염기 길이의 보편적인 프로브 세트를 어셈블리시키는 단계로 이루어진 방법.
  27. 제 19항에 있어서, 상기 노출 단계 또는 상기 인큐베이팅 단계가 6, 7 8, 9 또는 10 염기 길이의 보편적인 프로브 세트를 어셈블리시키는 단계로 이루어진 방법.
  28. 제 20항에 있어서, 상기 노출 단계 또는 상기 인큐베이팅 단계가 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 21, 22, 23, 24, 25, 26, 27, 28, 29 또는 30 염기 길이의 불완전 프로브 세트를 어셈블리시키는 단계로 이루어진 방법.
  29. 핵산 단편에 대한 접합접을 가지며, 소수성 부위에 의해 분할된 기질을 함유하는, 하이브리디제이션에 의한 핵산 분석 장치
  30. 제 20항에 있어서, 상기 배치 단계가 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 21, 22, 23, 24, 25, 26, 27, 28, 29 또는 30 염기 길이의 불완전 프로브 세트를 어셈블리시키는 단계로 이루어진 방법.
  31. 제 1항에 있어서, 2개 이상의 염기를 포함하는 중복된 핵산 서열을 갖는 2개 이상의 프로브들의 하이브리디제이션을 검정함으로써, 어떤 세그먼트 내의 2개 이상의 상기 염기들의 상대적인 순서를 확인하는 단계를 추가로 포함하는 방법.
  32. 샘플을 프로브 어레이에 도입하고; 주어진 어떠한 시간에서도, 다수의 샘플 분자들이 라이게이트된 프로브들과 회합되지 않도록 온도를 조정한 다음; 표지된 프로브를 혼합물에 첨가하고; 혼합물을 라이게이즈와 함께 인큐베이팅시킨 다음; 유리 프로브들을 제거하고; 라이게이션 생성물을 검색하는 단계들로 이루어진 뉴클레오티드 서열 분석 방법.
  33. 제 1항에 있어서, 원하는 결과를 개선시키기 위해 부가적인 프로브들을 정의하는 단계와 상기 노출, 인큐베이팅, 검색 및 분석 단계들을 반복하는 단계들을 추가로 포함하는 방법.
  34. 제 1항에 있어서, 상기 복수개의 핵산 세그먼트들을 재사용하기 위해 기질로부터 프로브들을 벗겨내는 단계를 추가로 포함하는 방법.
KR1019970703847A 1994-12-09 1995-12-08 디엔에이(dna) 시퀀싱 및 디엔에이(dna) 동정을 위한 방법 및 장치(methods and apparatus for dna sequencing and dna identification) Ceased KR980700433A (ko)

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