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  1. C. 医薬保健学域; 医学類・薬学類・医薬科学類・保健学類
  2. c 10. 学術雑誌掲載論文(医・保健)
  3. 1. 査読済論文(医学・保健)

Gene amplification of ESR1 in breast cancers-fact or fiction? A fluorescence in situ hybridization and multiplex ligation-dependent probe amplification study

http://hdl.handle.net/2297/30345
http://hdl.handle.net/2297/30345
3d46a807-c0e3-4ae7-b65e-dc79622a735f
名前 / ファイル ライセンス アクション
ME-PR-OOI-A-8.pdf ME-PR-OOI-A-8.pdf (799.2 kB)
Item type 学術雑誌論文 / Journal Article(1)
公開日 2017-10-03
タイトル
タイトル Gene amplification of ESR1 in breast cancers-fact or fiction? A fluorescence in situ hybridization and multiplex ligation-dependent probe amplification study
言語
言語 eng
資源タイプ
資源タイプ識別子 http://purl.org/coar/resource_type/c_6501
資源タイプ journal article
著者 Ooi, Akishi

× Ooi, Akishi

WEKO 245
e-Rad 50160411
金沢大学研究者情報 50160411
研究者番号 50160411

Ooi, Akishi

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Inokuchi, Masafumi

× Inokuchi, Masafumi

WEKO 508
金沢大学研究者情報 90401918
研究者番号 90401918

Inokuchi, Masafumi

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Harada, Shinichi

× Harada, Shinichi

WEKO 162
e-Rad 90272955
金沢大学研究者情報 90272955
研究者番号 90272955

Harada, Shinichi

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Inazawa, Johji

× Inazawa, Johji

WEKO 22900

Inazawa, Johji

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Tajiri, Ryousuke

× Tajiri, Ryousuke

WEKO 914
研究者番号 10402059

Tajiri, Ryousuke

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Sawada-Kitamura, Seiko

× Sawada-Kitamura, Seiko

WEKO 1009
研究者番号 20467103

Sawada-Kitamura, Seiko

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Ikeda, Hiroko

× Ikeda, Hiroko

WEKO 642
e-Rad 10447675
金沢大学研究者情報 10447675
研究者番号 10447675

Ikeda, Hiroko

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Kawashima, Hiroko

× Kawashima, Hiroko

WEKO 22901
金沢大学研究者情報 70293355
研究者番号 70293355

Kawashima, Hiroko

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Dobashi, Yoh

× Dobashi, Yoh

WEKO 22902

Dobashi, Yoh

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書誌情報 Journal of Pathology

巻 227, 号 1, p. 8-16, 発行日 2012-05-01
DOI
関連タイプ isVersionOf
識別子タイプ DOI
関連識別子 https://doi.org/10.1002/path.3974
出版者
出版者 John Wiley and Sons
抄録
内容記述タイプ Abstract
内容記述 Oestrogen receptor-alpha (ERα), encoded by the ESR1 gene located on 6q25, is a nuclear transcription factor. Since it was reported in 2007 that more than 20% of breast cancers show ESR1 gene amplification, there has been considerable controversy about its frequency and clinical significance. We set out to assess the frequency and levels of ESR1 amplification in breast cancers. In a total of 106 breast needle biopsy specimens examined by immunohistochemistry, 78 tumours contained more than 10% ERα-positive cancer cells. In fluorescence in situ hybridization (FISH) analysis with an ESR1-specific probe, variously extended ESR1 signals were found in ERα-expressing cells. Some of these were indistinguishable from large clustered signals generally accepted to mean high-level gene amplification in homogeneously staining regions (HSRs), and could be considered to represent gene amplification. However, with RNase treatment, the 'HSR-like' signals changed to small compact signals, and are thus thought to represent concentrated RNA. FISH using two differently labelled probes corresponding to the non-overlapping 5'- and 3'-end portions of the ESR1 gene on touch smears showed a preserved spatial relationship of the 3' to 5' sequence of ESR1, therefore strongly suggesting that the RNA consisted of primary transcripts. Using touch smears obtained from 51 fresh tumours, precise enumeration of ESR1 signals with a correction by the number of centromere 6 on FISH after RNase A treatment revealed that three tumours (5.9%) had tumour cells with one to three additional copies of ESR1 as predominant subpopulations. This infrequent and low level of gene amplification of ESR1 was also detected as a 'gain' of the gene by analysis with multiplex ligation-dependent probe amplification (MLPA). The consistent results from immunohistochemistry, FISH, and MLPA in the present study settle the long-standing debate concerning gene amplification of ESR1 in breast carcinoma. © 2012 Pathological Society of Great Britain and Ireland. Published by John Wiley & Sons, Ltd
著者版フラグ
出版タイプ AM
出版タイプResource http://purl.org/coar/version/c_ab4af688f83e57aa
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