Extraction and processing of high quality RNA from impalpable and macroscopically invisible prostate cancer for microarray gene expression analysis.

Thorsten Schlomm; Andreas M Luebke; Holger Sültmann; Olaf Hellwinkel; Ulrich Sauer; Annemarie Poustka; Kerstin A David; Felix K H Chun; Alexander Haese; Markus Graefen; Andreas Erbersdobler; Hartwig Huland

Extraction and processing of high quality RNA from impalpable and macroscopically invisible prostate cancer for microarray gene expression analysis.

Standard

Extraction and processing of high quality RNA from impalpable and macroscopically invisible prostate cancer for microarray gene expression analysis. / Schlomm, Thorsten; Luebke, Andreas M; Sültmann, Holger; Hellwinkel, Olaf; Sauer, Ulrich; Poustka, Annemarie; David, Kerstin A; Chun, Felix K H; Haese, Alexander; Graefen, Markus; Erbersdobler, Andreas; Huland, Hartwig.

In: INT J ONCOL, Vol. 27, No. 3, 3, 2005, p. 713-720.

Research output: SCORING: Contribution to journal › SCORING: Journal article › Research › peer-review

Harvard

Schlomm, T, Luebke, AM, Sültmann, H, Hellwinkel, O, Sauer, U, Poustka, A, David, KA, Chun, FKH, Haese, A, Graefen, M, Erbersdobler, A & Huland, H 2005, 'Extraction and processing of high quality RNA from impalpable and macroscopically invisible prostate cancer for microarray gene expression analysis.', INT J ONCOL, vol. 27, no. 3, 3, pp. 713-720. <http://www.ncbi.nlm.nih.gov/pubmed/16077921?dopt=Citation>

APA

Schlomm, T., Luebke, A. M., Sültmann, H., Hellwinkel, O., Sauer, U., Poustka, A., David, K. A., Chun, F. K. H., Haese, A., Graefen, M., Erbersdobler, A., & Huland, H. (2005). Extraction and processing of high quality RNA from impalpable and macroscopically invisible prostate cancer for microarray gene expression analysis. INT J ONCOL, 27(3), 713-720. [3]. http://www.ncbi.nlm.nih.gov/pubmed/16077921?dopt=Citation

Vancouver

Schlomm T, Luebke AM, Sültmann H, Hellwinkel O, Sauer U, Poustka A et al. Extraction and processing of high quality RNA from impalpable and macroscopically invisible prostate cancer for microarray gene expression analysis. INT J ONCOL. 2005;27(3):713-720. 3.

Bibtex

@article{30b83067d9204d8eb3f96ba3e8cc29fd,

title = "Extraction and processing of high quality RNA from impalpable and macroscopically invisible prostate cancer for microarray gene expression analysis.",

abstract = "Molecular analyses of early-stage prostate cancers are necessary to assess their potential clinical significance based on established and/or novel biomarkers for tailored clinical management. A prerequisite for the application of RNA-based analyses of such, mostly macroscopically-undetectable, small prostate carcinomas is the recovery and preservation of sufficient RNA quantities and quality. Furthermore, in prostate cancer, heterogeneity is a common phenomenon that includes a juxtaposition of different tissue compositions and variable histological grades within the same tumor focus. To better understand the molecular mechanisms of prostate cancer, it is essential to correlate molecular data with a specific cell type. Here, we present a tissue collecting protocol which is aligned with the preoperative evaluation of tumor localization. In combination with the technique of laser microdissection and pressure catapulting, we are able to preserve RNA of high quality from homogeneous cell populations of macroscopically-undetectable small prostate carcinomas. To obtain the necessary RNA quantities for whole genome cDNA microarrays, the isolated total RNAs were amplified by T7-based RNA-polymerase in vitro transcription. The microarray analyses (Human Unigene Set RZPD3.1) resulted in 216 differentially expressed genes (191 down-regulated, 25 up-regulated). Among these were several known prostate cancer relevant genes, such as AMACR, TARP, LIM, GPR160 (all up-regulated), CAV1, NTN1, MT1X; CLU, TRIM29, SPARCL1 and HSPB8 (all down-regulated).",

author = "Thorsten Schlomm and Luebke, {Andreas M} and Holger S{\"u}ltmann and Olaf Hellwinkel and Ulrich Sauer and Annemarie Poustka and David, {Kerstin A} and Chun, {Felix K H} and Alexander Haese and Markus Graefen and Andreas Erbersdobler and Hartwig Huland",

year = "2005",

language = "Deutsch",

volume = "27",

pages = "713--720",

journal = "INT J ONCOL",

issn = "1019-6439",

publisher = "Spandidos Publications",

number = "3",

}

RIS

TY - JOUR

T1 - Extraction and processing of high quality RNA from impalpable and macroscopically invisible prostate cancer for microarray gene expression analysis.

AU - Schlomm, Thorsten

AU - Luebke, Andreas M

AU - Sültmann, Holger

AU - Hellwinkel, Olaf

AU - Sauer, Ulrich

AU - Poustka, Annemarie

AU - David, Kerstin A

AU - Chun, Felix K H

AU - Haese, Alexander

AU - Graefen, Markus

AU - Erbersdobler, Andreas

AU - Huland, Hartwig

PY - 2005

Y1 - 2005

N2 - Molecular analyses of early-stage prostate cancers are necessary to assess their potential clinical significance based on established and/or novel biomarkers for tailored clinical management. A prerequisite for the application of RNA-based analyses of such, mostly macroscopically-undetectable, small prostate carcinomas is the recovery and preservation of sufficient RNA quantities and quality. Furthermore, in prostate cancer, heterogeneity is a common phenomenon that includes a juxtaposition of different tissue compositions and variable histological grades within the same tumor focus. To better understand the molecular mechanisms of prostate cancer, it is essential to correlate molecular data with a specific cell type. Here, we present a tissue collecting protocol which is aligned with the preoperative evaluation of tumor localization. In combination with the technique of laser microdissection and pressure catapulting, we are able to preserve RNA of high quality from homogeneous cell populations of macroscopically-undetectable small prostate carcinomas. To obtain the necessary RNA quantities for whole genome cDNA microarrays, the isolated total RNAs were amplified by T7-based RNA-polymerase in vitro transcription. The microarray analyses (Human Unigene Set RZPD3.1) resulted in 216 differentially expressed genes (191 down-regulated, 25 up-regulated). Among these were several known prostate cancer relevant genes, such as AMACR, TARP, LIM, GPR160 (all up-regulated), CAV1, NTN1, MT1X; CLU, TRIM29, SPARCL1 and HSPB8 (all down-regulated).

AB - Molecular analyses of early-stage prostate cancers are necessary to assess their potential clinical significance based on established and/or novel biomarkers for tailored clinical management. A prerequisite for the application of RNA-based analyses of such, mostly macroscopically-undetectable, small prostate carcinomas is the recovery and preservation of sufficient RNA quantities and quality. Furthermore, in prostate cancer, heterogeneity is a common phenomenon that includes a juxtaposition of different tissue compositions and variable histological grades within the same tumor focus. To better understand the molecular mechanisms of prostate cancer, it is essential to correlate molecular data with a specific cell type. Here, we present a tissue collecting protocol which is aligned with the preoperative evaluation of tumor localization. In combination with the technique of laser microdissection and pressure catapulting, we are able to preserve RNA of high quality from homogeneous cell populations of macroscopically-undetectable small prostate carcinomas. To obtain the necessary RNA quantities for whole genome cDNA microarrays, the isolated total RNAs were amplified by T7-based RNA-polymerase in vitro transcription. The microarray analyses (Human Unigene Set RZPD3.1) resulted in 216 differentially expressed genes (191 down-regulated, 25 up-regulated). Among these were several known prostate cancer relevant genes, such as AMACR, TARP, LIM, GPR160 (all up-regulated), CAV1, NTN1, MT1X; CLU, TRIM29, SPARCL1 and HSPB8 (all down-regulated).

M3 - SCORING: Zeitschriftenaufsatz

VL - 27

SP - 713

EP - 720

JO - INT J ONCOL

JF - INT J ONCOL

SN - 1019-6439

IS - 3

M1 - 3

ER -