Aromatase immunoreactivity is increased in mammographically dense regions of the breast

Celine M. Vachon; Hironobu Sasano; Karthik Ghosh; Kathleen R. Brandt; David A. Watson; Carol Reynolds; Wilma L. Lingle; Paul E. Goss; Rong Li; Sarah E. Aiyar; Christopher G. Scott; V. Shane Pankratz; Richard J. Santen; James N. Ingle

doi:10.1007/s10549-010-0944-6

Aromatase immunoreactivity is increased in mammographically dense regions of the breast

Celine M. Vachon, Hironobu Sasano, Karthik Ghosh, Kathleen R. Brandt, David A. Watson, Carol Reynolds, Wilma L. Lingle, Paul E. Goss, Rong Li, Sarah E. Aiyar, Christopher G. Scott, V. Shane Pankratz, Richard J. Santen, James N. Ingle

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Abstract

Mammographic breast density (MBD) is one of the strongest risk factors for breast cancer. Unfortunately, the biologic basis underlying this association is unknown. This study compared aromatase expression or immunoreactivity (IR) in core biopsies from mammographically dense versus non-dense regions of the breast to examine whether estrogen synthesis in the breast is associated with MBD and one possible mechanism through which MBD may influence breast cancer. Eligible participants were 40+ years, had a screening mammogram with visible MBD and no prior cancer or current endocrine therapy. Mammograms were used to identify dense and non-dense regions and ultrasound-guided core biopsies were performed to obtain tissue from these regions. Immunostaining for aromatase employed the streptavidin-biotin amplification method and #677 mouse monoclonal antibody. Aromatase IR was scored in terms of extent and intensity of staining for each cell type (stroma, epithelium, adipocytes) on histologic sections. A modified histological H-score provided quantitation of aromatase IR in each cell type and overall. Repeated measure analyses evaluated average differences (β_H) in H-score in dense versus non-dense tissue within and across cell types. Forty-nine women with mean age 50 years (range: 40-82), participated. Aromatase IR was increased in dense (vs. non-dense) tissue in both the stroma (β_H = 0.58) and epithelium (β_H = 0.12) (P < 0.01). Adipocytes from non-dense tissue, however, had a greater IR compared to those from dense tissue (β_H = -0.24, P < 0.01). An overall H-score which integrated results from all cell types demonstrated that aromatase IR was twice as great for dense (mean H-score = 0.90, SD = 0.53) versus non-dense (mean H-score = 0.45, SD = 0.39) breast tissue (β_H = 0.45; P < 0.001). Overall, aromatase IR was greater for mammographically dense versus non-dense tissue and may partly explain how MBD influences breast cancer.

Original language	English (US)
Pages (from-to)	243-252
Number of pages	10
Journal	Breast Cancer Research and Treatment
Volume	125
Issue number	1
DOIs	https://doi.org/10.1007/s10549-010-0944-6
State	Published - Jan 2011

Keywords

Aromatase
Breast density
Dense area

ASJC Scopus subject areas

Oncology
Cancer Research

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10.1007/s10549-010-0944-6

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Vachon, C. M., Sasano, H., Ghosh, K., Brandt, K. R., Watson, D. A., Reynolds, C., Lingle, W. L., Goss, P. E., Li, R., Aiyar, S. E., Scott, C. G., Pankratz, V. S., Santen, R. J., & Ingle, J. N. (2011). Aromatase immunoreactivity is increased in mammographically dense regions of the breast. Breast Cancer Research and Treatment, 125(1), 243-252. https://doi.org/10.1007/s10549-010-0944-6

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title = "Aromatase immunoreactivity is increased in mammographically dense regions of the breast",

abstract = "Mammographic breast density (MBD) is one of the strongest risk factors for breast cancer. Unfortunately, the biologic basis underlying this association is unknown. This study compared aromatase expression or immunoreactivity (IR) in core biopsies from mammographically dense versus non-dense regions of the breast to examine whether estrogen synthesis in the breast is associated with MBD and one possible mechanism through which MBD may influence breast cancer. Eligible participants were 40+ years, had a screening mammogram with visible MBD and no prior cancer or current endocrine therapy. Mammograms were used to identify dense and non-dense regions and ultrasound-guided core biopsies were performed to obtain tissue from these regions. Immunostaining for aromatase employed the streptavidin-biotin amplification method and #677 mouse monoclonal antibody. Aromatase IR was scored in terms of extent and intensity of staining for each cell type (stroma, epithelium, adipocytes) on histologic sections. A modified histological H-score provided quantitation of aromatase IR in each cell type and overall. Repeated measure analyses evaluated average differences (βH) in H-score in dense versus non-dense tissue within and across cell types. Forty-nine women with mean age 50 years (range: 40-82), participated. Aromatase IR was increased in dense (vs. non-dense) tissue in both the stroma (βH = 0.58) and epithelium (βH = 0.12) (P < 0.01). Adipocytes from non-dense tissue, however, had a greater IR compared to those from dense tissue (βH = -0.24, P < 0.01). An overall H-score which integrated results from all cell types demonstrated that aromatase IR was twice as great for dense (mean H-score = 0.90, SD = 0.53) versus non-dense (mean H-score = 0.45, SD = 0.39) breast tissue (βH = 0.45; P < 0.001). Overall, aromatase IR was greater for mammographically dense versus non-dense tissue and may partly explain how MBD influences breast cancer.",

keywords = "Aromatase, Breast density, Dense area",

author = "Vachon, {Celine M.} and Hironobu Sasano and Karthik Ghosh and Brandt, {Kathleen R.} and Watson, {David A.} and Carol Reynolds and Lingle, {Wilma L.} and Goss, {Paul E.} and Rong Li and Aiyar, {Sarah E.} and Scott, {Christopher G.} and Pankratz, {V. Shane} and Santen, {Richard J.} and Ingle, {James N.}",

note = "Funding Information: Acknowledgments We thank the participants in this study, who provided samples for investigations of the determinants of breast density. This study was financially supported by the Mayo Clinic Breast SPORE, NIH CA116201; NIH K12 RR24151 for the KL2 Clinical and Translational Science Award-Mentored Career Development Program; and Friends for an Earlier Breast Cancer Test.",

year = "2011",

month = jan,

doi = "10.1007/s10549-010-0944-6",

language = "English (US)",

volume = "125",

pages = "243--252",

journal = "Breast Cancer Research and Treatment",

issn = "0167-6806",

publisher = "Springer New York",

number = "1",

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TY - JOUR

T1 - Aromatase immunoreactivity is increased in mammographically dense regions of the breast

AU - Vachon, Celine M.

AU - Sasano, Hironobu

AU - Ghosh, Karthik

AU - Brandt, Kathleen R.

AU - Watson, David A.

AU - Reynolds, Carol

AU - Lingle, Wilma L.

AU - Goss, Paul E.

AU - Li, Rong

AU - Aiyar, Sarah E.

AU - Scott, Christopher G.

AU - Pankratz, V. Shane

AU - Santen, Richard J.

AU - Ingle, James N.

N1 - Funding Information: Acknowledgments We thank the participants in this study, who provided samples for investigations of the determinants of breast density. This study was financially supported by the Mayo Clinic Breast SPORE, NIH CA116201; NIH K12 RR24151 for the KL2 Clinical and Translational Science Award-Mentored Career Development Program; and Friends for an Earlier Breast Cancer Test.

PY - 2011/1

Y1 - 2011/1

N2 - Mammographic breast density (MBD) is one of the strongest risk factors for breast cancer. Unfortunately, the biologic basis underlying this association is unknown. This study compared aromatase expression or immunoreactivity (IR) in core biopsies from mammographically dense versus non-dense regions of the breast to examine whether estrogen synthesis in the breast is associated with MBD and one possible mechanism through which MBD may influence breast cancer. Eligible participants were 40+ years, had a screening mammogram with visible MBD and no prior cancer or current endocrine therapy. Mammograms were used to identify dense and non-dense regions and ultrasound-guided core biopsies were performed to obtain tissue from these regions. Immunostaining for aromatase employed the streptavidin-biotin amplification method and #677 mouse monoclonal antibody. Aromatase IR was scored in terms of extent and intensity of staining for each cell type (stroma, epithelium, adipocytes) on histologic sections. A modified histological H-score provided quantitation of aromatase IR in each cell type and overall. Repeated measure analyses evaluated average differences (βH) in H-score in dense versus non-dense tissue within and across cell types. Forty-nine women with mean age 50 years (range: 40-82), participated. Aromatase IR was increased in dense (vs. non-dense) tissue in both the stroma (βH = 0.58) and epithelium (βH = 0.12) (P < 0.01). Adipocytes from non-dense tissue, however, had a greater IR compared to those from dense tissue (βH = -0.24, P < 0.01). An overall H-score which integrated results from all cell types demonstrated that aromatase IR was twice as great for dense (mean H-score = 0.90, SD = 0.53) versus non-dense (mean H-score = 0.45, SD = 0.39) breast tissue (βH = 0.45; P < 0.001). Overall, aromatase IR was greater for mammographically dense versus non-dense tissue and may partly explain how MBD influences breast cancer.

AB - Mammographic breast density (MBD) is one of the strongest risk factors for breast cancer. Unfortunately, the biologic basis underlying this association is unknown. This study compared aromatase expression or immunoreactivity (IR) in core biopsies from mammographically dense versus non-dense regions of the breast to examine whether estrogen synthesis in the breast is associated with MBD and one possible mechanism through which MBD may influence breast cancer. Eligible participants were 40+ years, had a screening mammogram with visible MBD and no prior cancer or current endocrine therapy. Mammograms were used to identify dense and non-dense regions and ultrasound-guided core biopsies were performed to obtain tissue from these regions. Immunostaining for aromatase employed the streptavidin-biotin amplification method and #677 mouse monoclonal antibody. Aromatase IR was scored in terms of extent and intensity of staining for each cell type (stroma, epithelium, adipocytes) on histologic sections. A modified histological H-score provided quantitation of aromatase IR in each cell type and overall. Repeated measure analyses evaluated average differences (βH) in H-score in dense versus non-dense tissue within and across cell types. Forty-nine women with mean age 50 years (range: 40-82), participated. Aromatase IR was increased in dense (vs. non-dense) tissue in both the stroma (βH = 0.58) and epithelium (βH = 0.12) (P < 0.01). Adipocytes from non-dense tissue, however, had a greater IR compared to those from dense tissue (βH = -0.24, P < 0.01). An overall H-score which integrated results from all cell types demonstrated that aromatase IR was twice as great for dense (mean H-score = 0.90, SD = 0.53) versus non-dense (mean H-score = 0.45, SD = 0.39) breast tissue (βH = 0.45; P < 0.001). Overall, aromatase IR was greater for mammographically dense versus non-dense tissue and may partly explain how MBD influences breast cancer.

KW - Aromatase

KW - Breast density

KW - Dense area

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JO - Breast Cancer Research and Treatment

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ER -

Aromatase immunoreactivity is increased in mammographically dense regions of the breast

Abstract

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