Proteomic Analysis of High-Grade Dysplastic Cervical Cells Obtained from ThinPrep Slides Using Laser Capture Microdissection and Mass Spectrometry

Gu, Yuzong; Wu, Shiaw Lin; Meyer, Jane L.; Hancock, William S.; Burg, Lawrence J.; Linder, James; Hanlon, David; Karger, Barry L.

doi:10.1021/pr070319j

Cited by 44 publications

(45 citation statements)

References 29 publications

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“…In high-grade dysplastic cervical cells filamin, vimentin and vinculin were upregulated (Gu et al, 2007) in contrast to the findings in cancer cells in our study.…”

Section: Cytoskeletal Proteinscontrasting

confidence: 99%

Differential tissue-specific protein markers of vaginal carcinoma

et al. 2009

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The objective was to identify proteins differentially expressed in vaginal cancer to elucidate relevant cancer-related proteins. A total of 16 fresh-frozen tissue biopsies, consisting of 5 biopsies from normal vaginal epithelium, 6 from primary vaginal carcinomas and 5 from primary cervical carcinomas, were analysed using two-dimensional gel electrophoresis (2-DE) and MALDI-TOF mass spectrometry. Of the 43 proteins identified with significant alterations in protein expression between non-tumourous and tumourous tissue, 26 were upregulated and 17 were downregulated. Some were similarly altered in vaginal and cervical carcinoma, including cytoskeletal proteins, tumour suppressor proteins, oncoproteins implicated in apoptosis and proteins in the ubiquitin -proteasome pathway. Three proteins were uniquely altered in vaginal carcinoma (DDX48, erbB3-binding protein and biliverdin reductase) and five in cervical carcinoma (peroxiredoxin 2, annexin A2, sarcomeric tropomyosin kappa, human ribonuclease inhibitor and prolyl-4-hydrolase beta). The identified proteins imply involvement of multiple different cellular pathways in the carcinogenesis of vaginal carcinoma. Similar protein alterations were found between vaginal and cervical carcinoma suggesting common tumourigenesis. However, the expression level of some of these proteins markedly differs among the three tissue specimens indicating that they might be useful molecular markers.

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“…In high-grade dysplastic cervical cells filamin, vimentin and vinculin were upregulated (Gu et al, 2007) in contrast to the findings in cancer cells in our study.…”

Section: Cytoskeletal Proteinscontrasting

confidence: 99%

Differential tissue-specific protein markers of vaginal carcinoma

et al. 2009

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“…Laser capture microdissection is often used in conjunction with MS-based protein identification technology to assist with the discovery of tumor-associated molecules in tissue specimens containing various types of cells (27,31,(61)(62)(63)(64). However, relatively few studies have used these techniques to identify OSCC/HNSCC-associated proteins in tissue specimens from patients with OSCC/HNSCC (15,17,29).…”

Section: Discussionmentioning

confidence: 99%

Enhanced Interferon Signaling Pathway in Oral Cancer Revealed by Quantitative Proteome Analysis of Microdissected Specimens Using 16O/18O Labeling and Integrated Two-dimensional LC-ESI-MALDI Tandem MS

Chi

Lee

Chang

et al. 2009

Molecular & Cellular Proteomics

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“…Each gel section was separately subjected to in-gel tryptic digestion as described previously (24). Briefly, proteins were reduced and alkylated, and incubated with trypsin for 18 h at 37°C.…”

Section: Materials-ammoniummentioning

confidence: 99%

“…Using only the limited amount of material collected by LCM (60,000 cells), a proteomic profile of each sample was separately acquired by label-free proteomics using our previously developed platform for analysis of LCM samples (24). To the best of our knowledge, this is the most comprehensive global study that compares proteomic signatures of phenotypically normal and ERϩ invasive malignant breast epithelial cells in multiple individual samples.…”

mentioning

confidence: 99%

In Situ Proteomic Analysis of Human Breast Cancer Epithelial Cells Using Laser Capture Microdissection: Annotation by Protein Set Enrichment Analysis and Gene Ontology

Cha

Imieliński

Rejtar

et al. 2010

Molecular & Cellular Proteomics

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Breast cancer is a major health problem that each year affects the lives of millions of women worldwide. In 2008, in the United States alone, ϳ180,000 women were diagnosed with invasive breast carcinoma (1). The use of high-throughput gene expression technologies applied to the study of human breast cancer has lead to the discovery of the "intrinsic gene signatures" that stratify human breast cancers into four subtypes that correlate remarkably well with clinically recognized breast cancer subtypes (2-6). These subtypes include "HER2ϩ," "basal," and "luminal A," "luminal B" breast cancers. HER2ϩ tumors are most frequently estrogen receptor (ER)-1 , express proliferation genes, as well as Her-2 and other genes linked to this latter locus. The basal tumors are most commonly ER negative, progesterone receptor negative and Her-2 negative. The luminal A and luminal B tumors express luminal cytokeratins, the estrogen receptor (ER), and trans-acting T-cell-specific transcription factor (GATA3).The luminal breast cancers (both A and B subtypes) constitute ϳ70% of all human breast cancers diagnosed worldwide. In general, the luminal breast cancers are associated with favorable prognosis as compared with the HER2ϩ and basal subtypes. Nevertheless, luminal B tumors have a worse prognosis than luminal A tumors, and recent data suggest

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Proteomic Analysis of High-Grade Dysplastic Cervical Cells Obtained from ThinPrep Slides Using Laser Capture Microdissection and Mass Spectrometry

Cited by 44 publications

References 29 publications

Differential tissue-specific protein markers of vaginal carcinoma

Differential tissue-specific protein markers of vaginal carcinoma

Enhanced Interferon Signaling Pathway in Oral Cancer Revealed by Quantitative Proteome Analysis of Microdissected Specimens Using 16O/18O Labeling and Integrated Two-dimensional LC-ESI-MALDI Tandem MS

In Situ Proteomic Analysis of Human Breast Cancer Epithelial Cells Using Laser Capture Microdissection: Annotation by Protein Set Enrichment Analysis and Gene Ontology

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