Rapid detection of ras oncogenes in human tumors: applications to colon, esophageal, and gastric cancer

W. Jiang; S. M. Kahn; J. G. Guillem; S. H. Lu; I. B. Weinstein

Rapid detection of ras oncogenes in human tumors: applications to colon, esophageal, and gastric cancer

W. Jiang, S. M. Kahn, J. G. Guillem, S. H. Lu, I. B. Weinstein

Department of Surgery

Research output: Contribution to journal › Article › peer-review

290 Scopus citations

Abstract

We have developed a rapid, nonradioactive large scale method for the detection of ras oncogenes in human tumors. DNA is amplified by the polymerase chain reaction (PCR), and then digested with specific restriction enzymes to detect either endogenous or primer-mediated Restriction Fragment Length Polymorphisms (RFLPs). We report here that three of 15 colon tumors tested contain K-ras codon 12 aspartic acid mutations and one, along with the HCT 116 codon carcinoma cell line, contains a K-ras codon 13 aspartic acid mutation. On the other hand, we did not detect H- or K-ras codon 12 mutations or the K-ras codon 13 aspartic acid mutation in 25 esophageal and 27 gastric cardia tumors isolated from patients in Lin-xing County, China. By incorporating nucleotide substitutions in PCR primers, this method can be applied towards the rapid, non-radioactive screening of virtually any genetic disease caused by known point mutations.

Original language	English (US)
Pages (from-to)	923-928
Number of pages	6
Journal	Oncogene
Volume	4
Issue number	7
State	Published - 1989

All Science Journal Classification (ASJC) codes

Molecular Biology
Genetics
Cancer Research

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Cite this

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title = "Rapid detection of ras oncogenes in human tumors: applications to colon, esophageal, and gastric cancer",

abstract = "We have developed a rapid, nonradioactive large scale method for the detection of ras oncogenes in human tumors. DNA is amplified by the polymerase chain reaction (PCR), and then digested with specific restriction enzymes to detect either endogenous or primer-mediated Restriction Fragment Length Polymorphisms (RFLPs). We report here that three of 15 colon tumors tested contain K-ras codon 12 aspartic acid mutations and one, along with the HCT 116 codon carcinoma cell line, contains a K-ras codon 13 aspartic acid mutation. On the other hand, we did not detect H- or K-ras codon 12 mutations or the K-ras codon 13 aspartic acid mutation in 25 esophageal and 27 gastric cardia tumors isolated from patients in Lin-xing County, China. By incorporating nucleotide substitutions in PCR primers, this method can be applied towards the rapid, non-radioactive screening of virtually any genetic disease caused by known point mutations.",

author = "W. Jiang and Kahn, \{S. M.\} and Guillem, \{J. G.\} and Lu, \{S. H.\} and Weinstein, \{I. B.\}",

year = "1989",

language = "English (US)",

volume = "4",

pages = "923--928",

journal = "Oncogene",

issn = "0950-9232",

publisher = "Springer Nature",

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TY - JOUR

T1 - Rapid detection of ras oncogenes in human tumors

T2 - applications to colon, esophageal, and gastric cancer

AU - Jiang, W.

AU - Kahn, S. M.

AU - Guillem, J. G.

AU - Lu, S. H.

AU - Weinstein, I. B.

PY - 1989

Y1 - 1989

N2 - We have developed a rapid, nonradioactive large scale method for the detection of ras oncogenes in human tumors. DNA is amplified by the polymerase chain reaction (PCR), and then digested with specific restriction enzymes to detect either endogenous or primer-mediated Restriction Fragment Length Polymorphisms (RFLPs). We report here that three of 15 colon tumors tested contain K-ras codon 12 aspartic acid mutations and one, along with the HCT 116 codon carcinoma cell line, contains a K-ras codon 13 aspartic acid mutation. On the other hand, we did not detect H- or K-ras codon 12 mutations or the K-ras codon 13 aspartic acid mutation in 25 esophageal and 27 gastric cardia tumors isolated from patients in Lin-xing County, China. By incorporating nucleotide substitutions in PCR primers, this method can be applied towards the rapid, non-radioactive screening of virtually any genetic disease caused by known point mutations.

AB - We have developed a rapid, nonradioactive large scale method for the detection of ras oncogenes in human tumors. DNA is amplified by the polymerase chain reaction (PCR), and then digested with specific restriction enzymes to detect either endogenous or primer-mediated Restriction Fragment Length Polymorphisms (RFLPs). We report here that three of 15 colon tumors tested contain K-ras codon 12 aspartic acid mutations and one, along with the HCT 116 codon carcinoma cell line, contains a K-ras codon 13 aspartic acid mutation. On the other hand, we did not detect H- or K-ras codon 12 mutations or the K-ras codon 13 aspartic acid mutation in 25 esophageal and 27 gastric cardia tumors isolated from patients in Lin-xing County, China. By incorporating nucleotide substitutions in PCR primers, this method can be applied towards the rapid, non-radioactive screening of virtually any genetic disease caused by known point mutations.

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M3 - Article

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JO - Oncogene

JF - Oncogene

IS - 7

ER -

Rapid detection of ras oncogenes in human tumors: applications to colon, esophageal, and gastric cancer

Abstract

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