Tumor cell-specific BRCA1 and RASSF1A hypermethylation in serum, plasma, and peritoneal fluid from ovarian cancer patients

Inmaculada Ibanez De Caceres; Cristina Battagli; Manel Esteller; James G. Herman; Essel Dulaimi; Mitchell I. Edelson; Cynthia Bergman; Hormoz Ehya; Burton L. Eisenberg; Paul Cairns

doi:10.1158/0008-5472.CAN-04-1529

Tumor cell-specific BRCA1 and RASSF1A hypermethylation in serum, plasma, and peritoneal fluid from ovarian cancer patients

Inmaculada Ibanez De Caceres
, Cristina Battagli
, Manel Esteller
, James G. Herman
, Essel Dulaimi
, Mitchell I. Edelson
, Cynthia Bergman
, Hormoz Ehya
, Burton L. Eisenberg
, Paul Cairns

Pathology

Fox Chase Cancer Center
Biomedical Network on Rare Diseases (CIBERER)
Johns Hopkins University

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

276 Scopus citations

Abstract

Because existing surgical and management methods can consistently cure only early-stage ovarian cancer, novel strategies for early detection are required. Silencing of tumor suppressor genes such as p16^INK4a, VHL, and hMLH1 have established promoter hypermethylation as a common mechanism for tumor suppressor inactivation in human cancer and as a promising target for molecular detection in bodily fluids. Using sensitive methylation-specific PCR, we screened matched tumor, preoperative serum or plasma, and peritoneal fluid (washes or ascites) DNA obtained from 50 patients with ovarian or primary peritoneal tumors for hypermethylation status of the normally unmethylated BRCA1 and RAS association domain family protein 1A tumor suppressor genes. Hypermethylation of one or both genes was found in 34 tumor DNA (68%). Additional examination of one or more of the adenomatous polyposis coli, p14^ARF, p16^INK4a, or death associated protein-kinase tumor suppressor genes revealed hypermethylation in each of the remaining 16 tumor DNA, which extended diagnostic coverage to 100%. Hypermethylation was observed in all histologic cell types, grades, and stages of ovarian tumor examined. An identical pattern of gene hypermethylation was found in the matched serum DNA from 41 of 50 patients (82% sensitivity), including 13 of 17 cases of stage I disease. Hypermethylation was detected in 28 of 30 peritoneal fluid DNA from stage IC-IV patients, including 3 cases with negative or atypical cytology. In contrast, no hypermethylation was observed in nonneoplastic tissue, peritoneal fluid, or serum from 40 control women (100% specificity). We conclude that promoter hypermethylation is a common and relatively early event in ovarian tumorigenesis that can be detected in the serum DNA from patients with ovary-confined (stage IA or B) tumors and in cytologically negative peritoneal fluid. Analysis of tumor-specific hypermethylation in serum DNA may enhance early detection of ovarian cancer.

Original language	English
Pages (from-to)	6476-6481
Number of pages	6
Journal	Cancer Research
Volume	64
Issue number	18
DOIs	https://doi.org/10.1158/0008-5472.CAN-04-1529
State	Published - Sep 15 2004

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SDG 3 Good Health and Well-being

Keywords

Adolescent
Adult
Aged
Aged, 80 and over
Ascitic Fluid/genetics
DNA Methylation
DNA, Neoplasm/blood
Female
Genes, BRCA1
Humans
Middle Aged
Ovarian Neoplasms/blood
Tumor Suppressor Proteins/genetics

Access to Document

10.1158/0008-5472.CAN-04-1529

Cite this

@article{376a8a01f8014ba187ae223d16ead5e3,

title = "Tumor cell-specific BRCA1 and RASSF1A hypermethylation in serum, plasma, and peritoneal fluid from ovarian cancer patients",

abstract = "Because existing surgical and management methods can consistently cure only early-stage ovarian cancer, novel strategies for early detection are required. Silencing of tumor suppressor genes such as p16INK4a, VHL, and hMLH1 have established promoter hypermethylation as a common mechanism for tumor suppressor inactivation in human cancer and as a promising target for molecular detection in bodily fluids. Using sensitive methylation-specific PCR, we screened matched tumor, preoperative serum or plasma, and peritoneal fluid (washes or ascites) DNA obtained from 50 patients with ovarian or primary peritoneal tumors for hypermethylation status of the normally unmethylated BRCA1 and RAS association domain family protein 1A tumor suppressor genes. Hypermethylation of one or both genes was found in 34 tumor DNA (68\%). Additional examination of one or more of the adenomatous polyposis coli, p14ARF, p16INK4a, or death associated protein-kinase tumor suppressor genes revealed hypermethylation in each of the remaining 16 tumor DNA, which extended diagnostic coverage to 100\%. Hypermethylation was observed in all histologic cell types, grades, and stages of ovarian tumor examined. An identical pattern of gene hypermethylation was found in the matched serum DNA from 41 of 50 patients (82\% sensitivity), including 13 of 17 cases of stage I disease. Hypermethylation was detected in 28 of 30 peritoneal fluid DNA from stage IC-IV patients, including 3 cases with negative or atypical cytology. In contrast, no hypermethylation was observed in nonneoplastic tissue, peritoneal fluid, or serum from 40 control women (100\% specificity). We conclude that promoter hypermethylation is a common and relatively early event in ovarian tumorigenesis that can be detected in the serum DNA from patients with ovary-confined (stage IA or B) tumors and in cytologically negative peritoneal fluid. Analysis of tumor-specific hypermethylation in serum DNA may enhance early detection of ovarian cancer.",

keywords = "Adolescent, Adult, Aged, Aged, 80 and over, Ascitic Fluid/genetics, DNA Methylation, DNA, Neoplasm/blood, Female, Genes, BRCA1, Humans, Middle Aged, Ovarian Neoplasms/blood, Tumor Suppressor Proteins/genetics",

author = "\{De Caceres\}, \{Inmaculada Ibanez\} and Cristina Battagli and Manel Esteller and Herman, \{James G.\} and Essel Dulaimi and Edelson, \{Mitchell I.\} and Cynthia Bergman and Hormoz Ehya and Eisenberg, \{Burton L.\} and Paul Cairns",

year = "2004",

month = sep,

day = "15",

doi = "10.1158/0008-5472.CAN-04-1529",

language = "English",

volume = "64",

pages = "6476--6481",

journal = "Cancer Research",

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publisher = "American Association for Cancer Research Inc.",

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TY - JOUR

T1 - Tumor cell-specific BRCA1 and RASSF1A hypermethylation in serum, plasma, and peritoneal fluid from ovarian cancer patients

AU - De Caceres, Inmaculada Ibanez

AU - Battagli, Cristina

AU - Esteller, Manel

AU - Herman, James G.

AU - Dulaimi, Essel

AU - Edelson, Mitchell I.

AU - Bergman, Cynthia

AU - Ehya, Hormoz

AU - Eisenberg, Burton L.

AU - Cairns, Paul

PY - 2004/9/15

Y1 - 2004/9/15

N2 - Because existing surgical and management methods can consistently cure only early-stage ovarian cancer, novel strategies for early detection are required. Silencing of tumor suppressor genes such as p16INK4a, VHL, and hMLH1 have established promoter hypermethylation as a common mechanism for tumor suppressor inactivation in human cancer and as a promising target for molecular detection in bodily fluids. Using sensitive methylation-specific PCR, we screened matched tumor, preoperative serum or plasma, and peritoneal fluid (washes or ascites) DNA obtained from 50 patients with ovarian or primary peritoneal tumors for hypermethylation status of the normally unmethylated BRCA1 and RAS association domain family protein 1A tumor suppressor genes. Hypermethylation of one or both genes was found in 34 tumor DNA (68%). Additional examination of one or more of the adenomatous polyposis coli, p14ARF, p16INK4a, or death associated protein-kinase tumor suppressor genes revealed hypermethylation in each of the remaining 16 tumor DNA, which extended diagnostic coverage to 100%. Hypermethylation was observed in all histologic cell types, grades, and stages of ovarian tumor examined. An identical pattern of gene hypermethylation was found in the matched serum DNA from 41 of 50 patients (82% sensitivity), including 13 of 17 cases of stage I disease. Hypermethylation was detected in 28 of 30 peritoneal fluid DNA from stage IC-IV patients, including 3 cases with negative or atypical cytology. In contrast, no hypermethylation was observed in nonneoplastic tissue, peritoneal fluid, or serum from 40 control women (100% specificity). We conclude that promoter hypermethylation is a common and relatively early event in ovarian tumorigenesis that can be detected in the serum DNA from patients with ovary-confined (stage IA or B) tumors and in cytologically negative peritoneal fluid. Analysis of tumor-specific hypermethylation in serum DNA may enhance early detection of ovarian cancer.

AB - Because existing surgical and management methods can consistently cure only early-stage ovarian cancer, novel strategies for early detection are required. Silencing of tumor suppressor genes such as p16INK4a, VHL, and hMLH1 have established promoter hypermethylation as a common mechanism for tumor suppressor inactivation in human cancer and as a promising target for molecular detection in bodily fluids. Using sensitive methylation-specific PCR, we screened matched tumor, preoperative serum or plasma, and peritoneal fluid (washes or ascites) DNA obtained from 50 patients with ovarian or primary peritoneal tumors for hypermethylation status of the normally unmethylated BRCA1 and RAS association domain family protein 1A tumor suppressor genes. Hypermethylation of one or both genes was found in 34 tumor DNA (68%). Additional examination of one or more of the adenomatous polyposis coli, p14ARF, p16INK4a, or death associated protein-kinase tumor suppressor genes revealed hypermethylation in each of the remaining 16 tumor DNA, which extended diagnostic coverage to 100%. Hypermethylation was observed in all histologic cell types, grades, and stages of ovarian tumor examined. An identical pattern of gene hypermethylation was found in the matched serum DNA from 41 of 50 patients (82% sensitivity), including 13 of 17 cases of stage I disease. Hypermethylation was detected in 28 of 30 peritoneal fluid DNA from stage IC-IV patients, including 3 cases with negative or atypical cytology. In contrast, no hypermethylation was observed in nonneoplastic tissue, peritoneal fluid, or serum from 40 control women (100% specificity). We conclude that promoter hypermethylation is a common and relatively early event in ovarian tumorigenesis that can be detected in the serum DNA from patients with ovary-confined (stage IA or B) tumors and in cytologically negative peritoneal fluid. Analysis of tumor-specific hypermethylation in serum DNA may enhance early detection of ovarian cancer.

KW - Adolescent

KW - Adult

KW - Aged

KW - Aged, 80 and over

KW - Ascitic Fluid/genetics

KW - DNA Methylation

KW - DNA, Neoplasm/blood

KW - Female

KW - Genes, BRCA1

KW - Humans

KW - Middle Aged

KW - Ovarian Neoplasms/blood

KW - Tumor Suppressor Proteins/genetics

UR - https://www.scopus.com/pages/publications/4644271551

U2 - 10.1158/0008-5472.CAN-04-1529

DO - 10.1158/0008-5472.CAN-04-1529

M3 - Article

C2 - 15374957

SN - 0008-5472

VL - 64

SP - 6476

EP - 6481

JO - Cancer Research

JF - Cancer Research

IS - 18

ER -

Tumor cell-specific BRCA1 and RASSF1A hypermethylation in serum, plasma, and peritoneal fluid from ovarian cancer patients

Abstract

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Keywords

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