|
1. |
Analysis of Gastrinomas by Immunohistochemistry and In Situ Hybridization Histochemistry |
|
Diagnostic Molecular Pathology,
Volume 1,
Issue 3,
1992,
Page 155-164
Philip Perkins,
Michael McLeod,
Long Jin,
Atsuschi Fukuuchi,
Kyung Cho,
Norman Thompson,
Ricardo Lloyd,
Preview
|
PDF (963KB)
|
|
摘要:
Gastrinomas from 25 patients were examined by immunohistochemistry (IHC) and in situ hybridization histochemistry (ISH). Most patients (84%) presented with the Zollinger-Ellison syndrome. Six had multiple endocrine neoplasia type I (MEN-I). Twelve patients (48%) had duodenal primaries and 11 of 12 of these had metastases to regional lymph nodes and/or liver in spite of the small sizes of the primary tumors (mean size of 0.9 cm). Five patients had pancreatic gastrinomas and eight patients had metastatic tumor in regional lymph nodes or liver at surgery but a primary was not found. IHC and ISH analyses snowed that all cases were positive for gastrin protein and 24 of 25 (96%) expressed gastrin mRNA that was easily detected in formalin-fixed, paraffin-embedded tissue sections. Both benign and malignant tumors expressed a subunit of human chorionic gonadotropin protein (a-HCG). However, only malignant gastrinomas (29%) expressed adrenocorticotropic hormone protein or proopiomelanocortin (POMC) mRNA. ISH and Northern hybridization analysis revealed that chromogranin A mRNA was the most common member of the chromo-granin/secretogranin (Cg/Sg) family which was expressed in both benign and malignant gastrinomas. These results indicate that duodenal gastrinomas are common in both sporadic and MEN-1-associated cases, and small duodenal primaries may be associated with extensive regional lymph node and liver metastases. Expression of ACTH/ POMC protein and mRNA was consistently associated only with malignant gastrinomas while gastrin protein, gastrin mRNA and Cgs/Sgs mRNAs were readily detected in both benign and malignant gastrinomas.
ISSN:1052-9551
出版商:OVID
年代:1992
数据来源: OVID
|
2. |
Secretogranin II Expression in Ewing's Sarcomas and Primitive Neuroectodermal Tumors |
|
Diagnostic Molecular Pathology,
Volume 1,
Issue 3,
1992,
Page 165-172
A. Pagani,
R. Fischer-Colbrie,
B. Sanfilippo,
H. Winkler,
M. Cerrato,
G. BuSSOlati,
Preview
|
PDF (725KB)
|
|
摘要:
Production of chromogranins. the acidic components of the chromaffin granules regarded as specific neuroendocrine markers, was analyzed by immunocytochemistry and hybridization (Northern blotting and in situ hybridization) in primary lesions and cell lines of Ewing's sarcomas. primitive neuroectodermal tumors (PNETs), and neuroblastomas. Antibodies and probes specific for chromogranin A (CgA), chromogranin B (CgB), and secretogranin II (SgII) were used. Ewing s sarcomas and PNETs. unlike neuroblastomas, were negative for CgA and CgB. Two primary Ewing s sarcomas, one primary PNET (an Askin tumor), and one PNET cell line (TC32) were found to strongly express the SgII gene, as shown by the presence of specific mRNA. This result supports the hypothesis that some Ewing s sarcomas represent a most primitive form of neuroectodermal tumor; in addition, it indicates a diagnostic role of SgII in cases of Ewing s sarcomas and PNETs.
ISSN:1052-9551
出版商:OVID
年代:1992
数据来源: OVID
|
3. |
A Simplified Method of Detection of Clonal Rearrangements of the T‐Cell Receptor-γ Chain Gene |
|
Diagnostic Molecular Pathology,
Volume 1,
Issue 3,
1992,
Page 173-179
Keith McCarthy,
John Sloane,
Janusz Kabarowski,
Estela Matutes,
Leanne Wiedemann,
Preview
|
PDF (576KB)
|
|
摘要:
A series of T-cell proliferations in peripheral blood, bone marrow, or tissue samples, together with seven T-cell lines, were analysed for clonality. The technique used employs the polymerase chain reaction (PCR) to amplify rearranged T-cell receptor 7 genes, using primers recognising conserved sequences in the variable and joining gene segments. Of the 20 cases of T-cell leukaemia or lymphoma analysed, a clone was detected in 14 (70%): Of seven T-cell lines, a clone was detected in 6 (84%). No positive results were recorded in eight non-T-cell disorders (including nonlymphoid malignancies and reactive disorders). When the results of this technique were combined with the results of our previously published method for the detection of clonally rearranged T-cell receptor-β (TCR-β) genes using PCR. 9 of 10 (90%) T-cell tumours were detected. This method uses only four primer combinations in two tubes, and is therefore simple and rapid: it requires no radiolabelling, uses only a small amount of tissue, and can be performed on formalin-fixed, paraffin-embedded tissue.
ISSN:1052-9551
出版商:OVID
年代:1992
数据来源: OVID
|
4. |
DNA Content Measurement and In Situ Hybridization in Condylomatous Cervical Lesions |
|
Diagnostic Molecular Pathology,
Volume 1,
Issue 3,
1992,
Page 180-184
Christine Clavel,
Laurent Zerat,
Isabelle Binninger,
Marie-Claude Boutterin,
Myriam Polette,
Joseph Monsonego,
Philippe Birembaut,
Preview
|
PDF (443KB)
|
|
摘要:
The present study reports results obtained with DNA ploidy measurement by Feulgen cytophotometry and in situ hybridization (ISH) on the same sections of 36 cervical lesions containing human papillomavirus (HPV) DNA. Fifteen of 16 low grade lesions [11 flat condylomas and five condylomatous with intraepithelial neoplasias (CIN)-1, 1 with condylomatous features] were diploid. “Oncogenic” HPV (types 16 and 33) were detected in three of these cases, while the aneuploid case expressed HPV type 11. By contrast, in the 12 CIN-2 and eight CIN-3 with condylomas, there was a good correlation between presence of an aneuploid DNA pattern and detection of “oncogenic” HPVs. Demonstration of an aneuploid profile and “oncogenic” HPV as found in all our CIN-3, may be indicative of a poor prognosis in low grade lesions. Hence, the combination of the two techniques (ISH and Feulgen cytophotometry) may provide significant prognostic information for condylomas and CINs.
ISSN:1052-9551
出版商:OVID
年代:1992
数据来源: OVID
|
5. |
Rapid Detection and Species Identification of Mycobacteria in Paraffin‐Embedded Tissues by Polymerase Chain Reaction |
|
Diagnostic Molecular Pathology,
Volume 1,
Issue 3,
1992,
Page 185-191
Ronald Ghossein,
Donald Ross,
Robert Salomon,
Arthur Rabson,
Preview
|
PDF (656KB)
|
|
摘要:
The sensitivity and specificity of the polymerase chain reaction (PCR) in the detection of mycobacteria in paraffin-embedded tissues and in crude lysates of mycobacterial cultures were assessed. Sections of formalin-fixed, paraffin-embedded tissues were deparaffinized and then subjected to a simple proteinase K and boiling lysis procedure. These preparations were used directly for PCR amplification of the 383 bp segment of the gene encoding the 65 kDa mycobacterial surface antigen. Crude lysates of mycobacteria were used as positive controls. The specificity of the PCR products was confirmed by Southern blot using a region-specific digoxigenin-labeled oligonucleotide probe and chemiluminescent detection. The 383 bp diagnostic fragment was visualized in 11 of 12 acid-fast bacilli (AFB) stain/culture-proven-positive blocks. Crude lysates of mycobacteria were detected to a sensitivity of approximately 80 organisms. Amplified fragments from paraffin-embedded tissues and mycobacterial cultures ofM. tuberculosis, M. avium-intracellulare, and saprophytic mycobacteria were distinguished by digestion with Nar 1 restriction endonuclease. These results suggest that PCR amplification followed by restriction enzyme digestion of the PCR product is a rapid, specific, and highly sensitive technique for the detection and speciation of mycobacteria in paraffin-embedded tissues.
ISSN:1052-9551
出版商:OVID
年代:1992
数据来源: OVID
|
6. |
An Approach to Definition of Genetic Alterations in Prostate Cancer |
|
Diagnostic Molecular Pathology,
Volume 1,
Issue 3,
1992,
Page 192-199
Sandra Wolman,
Jill Macoska,
Mark Micale,
Wael Sakr,
Preview
|
PDF (713KB)
|
|
摘要:
Growth patterns in prostatic cancer can reduce detect-ability of genetic alterations. Tumors show histologic grade heterogeneity, multifocality, interdigitation of benign and malignant glands, and varying amounts of stroma. These characteristics introduce sampling errors when one uses traditional methods for genetic analysis that depend on disaggregated cells [metaphase or interphase chromosome studies] or on tissue extracts [Southern blotting or polymerase chain reaction (PCR)] to detect molecular events. To circumvent these problems, we used two approaches to study paraffin-embedded tumors, which permit focused analysis of critical tissue components. Serial 4− to 5-μm sections are applied to slides in groups of three. Every second slide is hematoxylin and eosin stained to visualize areas of carcinoma, dysplasia. hyperplasia, and stroma; tumor-rich areas are circled with ink and used as templates to examine or excise the same areas from adjacent nonstained sections. PCR methods for quantitative and qualitative gene assay are effective in evaluating samples when alteration at a particular locus is suspected. Fluorescence in situ hybridization with chromosome-specific paracentromeric probes for detection of copy number of the relevant chromosome is applied to the adjacent section. Normal chromosome controls for both methods were demonstrated. This protocol enables us to correlate genetic alterations precisely with tumor extent and morphology.
ISSN:1052-9551
出版商:OVID
年代:1992
数据来源: OVID
|
7. |
Expression of Stromelysin 3 in the Stromal Elements of Human Basal Cell Carcinoma |
|
Diagnostic Molecular Pathology,
Volume 1,
Issue 3,
1992,
Page 200-205
Stephan Wagner,
Christine Ruhri,
Kerstin Kunth,
Brigitte Holecek,
Manfred Goos,
Heinz Hofler,
Michael Atkinson,
Preview
|
PDF (614KB)
|
|
摘要:
In basal cell carcinoma, release of proteolytic activity is implicated in extracellular matrix degradation and tumor infiltration. The stromelysin metalloproteinase family is a major candidate for the matrix proteolytic activity in infiltrative tumors. However, in murine models of basal cell carcinoma, neither stromelysin 1 nor 2 appears to play a role in tumor infiltration. We have analyzed the expression of the newly described stromelysin 3 in human basal cell carcinoma using Northern blot analysis and in situ hybridization. In 12 of 14 cases, levels of stromelysin 3 expression were more than tenfold above those observed in normal skin. In one of five cases of squamous cell carcinoma, stromelysin 3 expression was tenfold above levels seen in normal skin. Stromelysin 3 expression was either undetectable or extremely weak in all five cases of infiltrative malignant melanoma. In basal cell carcinoma, stromelysin 3 transcripts were localized by in situ hybridization to the stromal tissue immediately adjacent to basal cell carcinoma, the tumor cells themselves being negative. Therefore, expression of stromelysin 3 in stromal cells may be expected to play a significant role in destruction of the basal membrane zone and extracellular matrix in basal cell carcinoma invasion.
ISSN:1052-9551
出版商:OVID
年代:1992
数据来源: OVID
|
8. |
Molecular Pathology of Paraffin‐Embedded Tissue Current Clinical Applications |
|
Diagnostic Molecular Pathology,
Volume 1,
Issue 3,
1992,
Page 206-211
Carolyn Mies,
Preview
|
PDF (562KB)
|
|
摘要:
Molecular biology techniques have been adapted to analyze paraffin-embedded tissues, expanding their potential clinical utility. The isolation of intact nucleic acids from tissue blocks is fundamental to the molecular pathology of paraffin-embedded tissues. In vitro amplification with the polymerase chain reaction (PCR) promises to be the most useful means of retrospective analysis since it can be performed successfully on DNA that has partially degraded during fixation, paraffin embedding, and the extraction process. Four clinical situations in which DNA analysis of paraffin-embedded tissues can be helpful are: (a) gene rearrangement analysis in lymphoproliferative disorders, where fresh tissue has not been obtained at the time of surgery; (b) identification of infectious agents, particularly viruses; (c) genetic testing of families with a putative inherited disease where the affected member has died; and (d) specimen identification. The PCR and other techniques of genetic analysis are powerful in sensitivity and specificity when performed and interpreted with appropriate precautions and controls. DNA analysis of paraffin-embedded tissues will likely become a fixed part of the future pathologist's diagnostic armamentarium.
ISSN:1052-9551
出版商:OVID
年代:1992
数据来源: OVID
|
9. |
Localization ofMycobacterium Avium‐IntracellulareWithin a Skin Lesion of Bacillary Angiomatosis in a Patient with AIDS |
|
Diagnostic Molecular Pathology,
Volume 1,
Issue 3,
1992,
Page 212-216
Paul Sagerman,
David Relman,
Farhad Niroomand,
G. Niedt,
Preview
|
PDF (455KB)
|
|
摘要:
We report a 39-year-old man who had AIDS and who presented with an unusual cutaneous vascular lesion, which was clinically thought to be Kaposi's sarcoma. Histologically, the lesion was characterized by capillary proliferation and a mixed inflammatory infiltrate that included numerous histiocytes. The lesion was found to contain slender intracellular acid-fast bacilli, as well as plump extracellular Warthin-Starry-positive bacilli. The acid-fast bacilli were confirmed to beMycobacterium avium-intracellulareby subsequent positive blood cultures for this organism. To further investigate the lesion. polymerase chain reaction DNA amplification and sequencing was performed, and the lesion was found to contain DNA sequences identical to those previously established for the agent of bacillary angiomatosis. The lesion is thought to represent a lesion of bacillary angiomatosis with secondary involvement byM. avium-intracellulare.
ISSN:1052-9551
出版商:OVID
年代:1992
数据来源: OVID
|
10. |
Glossary |
|
Diagnostic Molecular Pathology,
Volume 1,
Issue 3,
1992,
Page 217-220
Preview
|
PDF (154KB)
|
|
ISSN:1052-9551
出版商:OVID
年代:1992
数据来源: OVID
|
|