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Hypomethylation of CYP11B2 in Aldosterone-Producing Adenoma
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The purpose of this study was to evaluate the DNA methylation levels of steroidogenic enzyme genes in aldosterone-producing adenoma (APA) and the effects of gene mutations in APA on the DNA methylation levels. DNA methylation array analysis was conducted using nonfunctioning adrenocortical adenoma (n=12) and APA (n=35) samples, including some with a
KCNJ5
mutation (n=21), an
ATP1A1
mutation (n=5), and without the known mutations (n=9). The quantitative polymerase chain reaction assay was performed for the detection of CYP11B2 and CYP11B1 expression levels in nonfunctioning adrenocortical adenoma and APA. We introduced the KCNJ5 T158A mutation using lentivirus delivery in the human adrenocortical 15 cell line, and analyzed the effects of the mutation on DNA methylation levels. We analyzed the 83 presumed DNA methylation sites of steroidogenic enzymes. In APA, we found 7 hypomethylated sites in
CYP11B2
and 1 hypomethylated and 6 hypermethylated sites in
CYP11B1
. There were no differences in the steroidogenic enzymes gene DNA methylation of peripheral leukocytes between nonfunctioning adrenocortical adenoma and APA. No
CYP11B2
methylation level was associated with CYP11B2 transcription levels in APA. All methylation sites, except for a CYP11B2 region, showed no difference among APAs with or without gene mutations. Human adrenocortical 15 cells with the KCNJ5 mutation showed no changes in
CYP11B2
or
CYP11B1
methylation levels compared with control cells. We demonstrated that
CYP11B2
in APA was extensively hypomethylated, and
CYP11B2
methylation in the region with hypomethylation was not induced by
KCNJ5
or
ATP1A1
mutations that cause aldosterone overproduction in APA and a
KCNJ5
mutation human adrenocortical 15 cells.
Ovid Technologies (Wolters Kluwer Health)
Title: Hypomethylation of CYP11B2 in Aldosterone-Producing Adenoma
Description:
The purpose of this study was to evaluate the DNA methylation levels of steroidogenic enzyme genes in aldosterone-producing adenoma (APA) and the effects of gene mutations in APA on the DNA methylation levels.
DNA methylation array analysis was conducted using nonfunctioning adrenocortical adenoma (n=12) and APA (n=35) samples, including some with a
KCNJ5
mutation (n=21), an
ATP1A1
mutation (n=5), and without the known mutations (n=9).
The quantitative polymerase chain reaction assay was performed for the detection of CYP11B2 and CYP11B1 expression levels in nonfunctioning adrenocortical adenoma and APA.
We introduced the KCNJ5 T158A mutation using lentivirus delivery in the human adrenocortical 15 cell line, and analyzed the effects of the mutation on DNA methylation levels.
We analyzed the 83 presumed DNA methylation sites of steroidogenic enzymes.
In APA, we found 7 hypomethylated sites in
CYP11B2
and 1 hypomethylated and 6 hypermethylated sites in
CYP11B1
.
There were no differences in the steroidogenic enzymes gene DNA methylation of peripheral leukocytes between nonfunctioning adrenocortical adenoma and APA.
No
CYP11B2
methylation level was associated with CYP11B2 transcription levels in APA.
All methylation sites, except for a CYP11B2 region, showed no difference among APAs with or without gene mutations.
Human adrenocortical 15 cells with the KCNJ5 mutation showed no changes in
CYP11B2
or
CYP11B1
methylation levels compared with control cells.
We demonstrated that
CYP11B2
in APA was extensively hypomethylated, and
CYP11B2
methylation in the region with hypomethylation was not induced by
KCNJ5
or
ATP1A1
mutations that cause aldosterone overproduction in APA and a
KCNJ5
mutation human adrenocortical 15 cells.
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