Expression, regulation and function of epithelial-stromal interaction 1 (breast), EPSTI1

René Villadsen; Helga Lind Nielsen; Fritz Rank; Ole William Petersen; Lone Rønnov-Jessen; Michala De Neergaard

Expression, regulation and function of epithelial-stromal interaction 1 (breast), EPSTI1

René Villadsen, Helga Lind Nielsen, Fritz Rank, Ole William Petersen, Lone Rønnov-Jessen, Michala De Neergaard

Cellebiologi og Fysiologi

Abstract

The transcript of epithelial-stromal interaction 1 (breast), EPSTI1, was originally found to be upregulated in invasive breast carcinomas as compared to normal breast tissue (Genomics 79:703, 2002). In the present study we investigated the expression, regulation and possible function of the protein product, EPSTI1. By use of a monoclonal antibody raised against a NH2-terminal peptide sequence the expression of native EPSTI1 was first analyzed by immunohistochemistry on tissue sections. EPSTI1 was primarily localized to the nucleus of both carcinoma and stromal cells with the highest expression in epithelial cells in close contact with stromal cells. Furthermore, preliminary data indicate that the expression was highest in estrogen receptor negative tumors. By comparison, in normal breast EPSTI1 was expressed primarily in the acini. To address a possible function of the protein we used a human breast epithelial cancer cell line, MCF-7, transfected with pRev-Tet-Off and pRevTRE with a FLAG-EPSTI1 insert. When cultured in 3-dimensional assays, the EPSTI1 expressing cells gave rise to more compact structures than the non-expressing cells, which resulted in loosely arranged/hollow structures. Immunocytochemistry indicated that EPSTI1 expressing cells also show elevated levels of STAT1 and á2â1-integrin, both of which have been implicated in the innate immune response. To investigate if EPSTI1 belongs to the group of interferon-response genes as suggested by others (Genome Biology 8:R191, 2007), we performed immunocytochemistry on a human breast epithelial cell line exposed to interferon-a. EPSTI1 as well as STAT1 were induced. Specific downregulation of EPSTI1 message with siRNAs also led to lower expression of á2â1-integrin. In conclusion, we have confirmed the existence of a protein product of EPSTI1 that is highly expressed in breast carcinomas at the epithelial-stromal interface as compared to normal breast. Furthermore, EPSTI1 is induced in response to interferon and may be involved in tissue organization.

Originalsprog	Engelsk
Tidsskrift	Acta Pathologica Microbiologica et Immunologica Scandinavica
Udgave nummer	5
Sider (fra-til)	430-431
Antal sider	1
ISSN	0903-4641
Status	Udgivet - 2008
Begivenhed	Danish Society for Cancer Research, 21st Annual Meeting - , Danmark Varighed: 30 apr. 2008 → 30 apr. 2008 Konferencens nummer: 21

Konference

Konference	Danish Society for Cancer Research, 21st Annual Meeting
Nummer	21
Land/Område	Danmark
Periode	30/04/2008 → 30/04/2008

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Citationsformater

Villadsen, R., Lind Nielsen, H., Rank, F., Petersen, O. W., Rønnov-Jessen, L., & Neergaard, M. D. (2008). Expression, regulation and function of epithelial-stromal interaction 1 (breast), EPSTI1. Acta Pathologica Microbiologica et Immunologica Scandinavica, (5), 430-431. http://www.ingentaconnect.com/content/mksg/apm/2008/00000116/00000005/art00050;jsessionid=gpok1qauw6ub.alexandra?format=print

Villadsen, R, Lind Nielsen, H, Rank, F, Petersen, OW, Rønnov-Jessen, L & Neergaard, MD 2008, 'Expression, regulation and function of epithelial-stromal interaction 1 (breast), EPSTI1', Acta Pathologica Microbiologica et Immunologica Scandinavica, nr. 5, s. 430-431. <http://www.ingentaconnect.com/content/mksg/apm/2008/00000116/00000005/art00050;jsessionid=gpok1qauw6ub.alexandra?format=print>

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title = "Expression, regulation and function of epithelial-stromal interaction 1 (breast), EPSTI1",

abstract = "The transcript of epithelial-stromal interaction 1 (breast), EPSTI1, was originally found to be upregulated in invasive breast carcinomas as compared to normal breast tissue (Genomics 79:703, 2002). In the present study we investigated the expression, regulation and possible function of the protein product, EPSTI1. By use of a monoclonal antibody raised against a NH2-terminal peptide sequence the expression of native EPSTI1 was first analyzed by immunohistochemistry on tissue sections. EPSTI1 was primarily localized to the nucleus of both carcinoma and stromal cells with the highest expression in epithelial cells in close contact with stromal cells. Furthermore, preliminary data indicate that the expression was highest in estrogen receptor negative tumors. By comparison, in normal breast EPSTI1 was expressed primarily in the acini. To address a possible function of the protein we used a human breast epithelial cancer cell line, MCF-7, transfected with pRev-Tet-Off and pRevTRE with a FLAG-EPSTI1 insert. When cultured in 3-dimensional assays, the EPSTI1 expressing cells gave rise to more compact structures than the non-expressing cells, which resulted in loosely arranged/hollow structures. Immunocytochemistry indicated that EPSTI1 expressing cells also show elevated levels of STAT1 and {\'a}2{\^a}1-integrin, both of which have been implicated in the innate immune response. To investigate if EPSTI1 belongs to the group of interferon-response genes as suggested by others (Genome Biology 8:R191, 2007), we performed immunocytochemistry on a human breast epithelial cell line exposed to interferon-a. EPSTI1 as well as STAT1 were induced. Specific downregulation of EPSTI1 message with siRNAs also led to lower expression of {\'a}2{\^a}1-integrin. In conclusion, we have confirmed the existence of a protein product of EPSTI1 that is highly expressed in breast carcinomas at the epithelial-stromal interface as compared to normal breast. Furthermore, EPSTI1 is induced in response to interferon and may be involved in tissue organization.",

author = "Ren{\'e} Villadsen and {Lind Nielsen}, Helga and Fritz Rank and Petersen, {Ole William} and Lone R{\o}nnov-Jessen and Neergaard, {Michala De}",

note = "Subject Category: Immunology; Microbiology; Pathology; Danish Society for Cancer Research, 21st Annual Meeting ; Conference date: 30-04-2008 Through 30-04-2008",

year = "2008",

language = "English",

pages = "430--431",

journal = "APMIS. Supplementum",

issn = "0903-465X",

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number = "5",

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TY - ABST

T1 - Expression, regulation and function of epithelial-stromal interaction 1 (breast), EPSTI1

AU - Villadsen, René

AU - Lind Nielsen, Helga

AU - Rank, Fritz

AU - Petersen, Ole William

AU - Rønnov-Jessen, Lone

AU - Neergaard, Michala De

N1 - Conference code: 21

PY - 2008

Y1 - 2008

N2 - The transcript of epithelial-stromal interaction 1 (breast), EPSTI1, was originally found to be upregulated in invasive breast carcinomas as compared to normal breast tissue (Genomics 79:703, 2002). In the present study we investigated the expression, regulation and possible function of the protein product, EPSTI1. By use of a monoclonal antibody raised against a NH2-terminal peptide sequence the expression of native EPSTI1 was first analyzed by immunohistochemistry on tissue sections. EPSTI1 was primarily localized to the nucleus of both carcinoma and stromal cells with the highest expression in epithelial cells in close contact with stromal cells. Furthermore, preliminary data indicate that the expression was highest in estrogen receptor negative tumors. By comparison, in normal breast EPSTI1 was expressed primarily in the acini. To address a possible function of the protein we used a human breast epithelial cancer cell line, MCF-7, transfected with pRev-Tet-Off and pRevTRE with a FLAG-EPSTI1 insert. When cultured in 3-dimensional assays, the EPSTI1 expressing cells gave rise to more compact structures than the non-expressing cells, which resulted in loosely arranged/hollow structures. Immunocytochemistry indicated that EPSTI1 expressing cells also show elevated levels of STAT1 and á2â1-integrin, both of which have been implicated in the innate immune response. To investigate if EPSTI1 belongs to the group of interferon-response genes as suggested by others (Genome Biology 8:R191, 2007), we performed immunocytochemistry on a human breast epithelial cell line exposed to interferon-a. EPSTI1 as well as STAT1 were induced. Specific downregulation of EPSTI1 message with siRNAs also led to lower expression of á2â1-integrin. In conclusion, we have confirmed the existence of a protein product of EPSTI1 that is highly expressed in breast carcinomas at the epithelial-stromal interface as compared to normal breast. Furthermore, EPSTI1 is induced in response to interferon and may be involved in tissue organization.

AB - The transcript of epithelial-stromal interaction 1 (breast), EPSTI1, was originally found to be upregulated in invasive breast carcinomas as compared to normal breast tissue (Genomics 79:703, 2002). In the present study we investigated the expression, regulation and possible function of the protein product, EPSTI1. By use of a monoclonal antibody raised against a NH2-terminal peptide sequence the expression of native EPSTI1 was first analyzed by immunohistochemistry on tissue sections. EPSTI1 was primarily localized to the nucleus of both carcinoma and stromal cells with the highest expression in epithelial cells in close contact with stromal cells. Furthermore, preliminary data indicate that the expression was highest in estrogen receptor negative tumors. By comparison, in normal breast EPSTI1 was expressed primarily in the acini. To address a possible function of the protein we used a human breast epithelial cancer cell line, MCF-7, transfected with pRev-Tet-Off and pRevTRE with a FLAG-EPSTI1 insert. When cultured in 3-dimensional assays, the EPSTI1 expressing cells gave rise to more compact structures than the non-expressing cells, which resulted in loosely arranged/hollow structures. Immunocytochemistry indicated that EPSTI1 expressing cells also show elevated levels of STAT1 and á2â1-integrin, both of which have been implicated in the innate immune response. To investigate if EPSTI1 belongs to the group of interferon-response genes as suggested by others (Genome Biology 8:R191, 2007), we performed immunocytochemistry on a human breast epithelial cell line exposed to interferon-a. EPSTI1 as well as STAT1 were induced. Specific downregulation of EPSTI1 message with siRNAs also led to lower expression of á2â1-integrin. In conclusion, we have confirmed the existence of a protein product of EPSTI1 that is highly expressed in breast carcinomas at the epithelial-stromal interface as compared to normal breast. Furthermore, EPSTI1 is induced in response to interferon and may be involved in tissue organization.

M3 - Conference abstract in journal

SN - 0903-465X

SP - 430

EP - 431

JO - APMIS. Supplementum

JF - APMIS. Supplementum

IS - 5

T2 - Danish Society for Cancer Research, 21st Annual Meeting

Y2 - 30 April 2008 through 30 April 2008

ER -

Expression, regulation and function of epithelial-stromal interaction 1 (breast), EPSTI1

Abstract

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