首页   按字顺浏览 期刊浏览 卷期浏览 Monoclonality in Gastric Lymphoma Detected in Formalin‐fixed, Paraffin&hyp...
Monoclonality in Gastric Lymphoma Detected in Formalin‐fixed, Paraffin‐embedded Endoscopic Biopsy Specimens Using Immunohistochemistry, In Situ Hybridization, and Polymerase Chain Reaction

 

作者: Hiroshi Inagaki,   Masaru Nonaka,   Seizo Nagaya,   Hisashi Tateyama,   Makoto Sasaki,   Tadaaki Eimoto,  

 

期刊: Diagnostic Molecular Pathology  (OVID Available online 1995)
卷期: Volume 4, issue 1  

页码: 32-38

 

ISSN:1052-9551

 

年代: 1995

 

出版商: OVID

 

关键词: Malignant lymphoma;Stomach;Immuno histochemistry;In situ hybridization;Immunoglobulin light-chain;Polymerase chain reaction;Gene rearrangement.

 

数据来源: OVID

 

摘要:

Diagnosis of gastric malignant lymphoma remains a challenge, especially when the tissue source is endoscopic biopsy specimens. Once an atypical lymphoid infiltrate is found, demonstration of clonality is the key to establishing a diagnosis of the disease. For this purpose, we evaluated the usefulness of immunohistochemistry, in situ hybridization, and polymerase chain reaction (PCR) using formalin-fixed, paraffin-embedded endoscopic materials from 20 patients with B-cell malignant lymphomas. Template DNA for PCR was obtained by microdissecting Giemsa-stained sections using a serial hematoxylin and eosin section as a guide. Clonal rearrangement bands were demonstrated in 15 of 20 cases (75%) by PCR, whereas expression of monotypic light-chain mRNA was detected in seven of 20 (35%) by in situ hybridization and monotypic light-chain restriction in four of 20 (20%) by conventional immunohistochemistry. Although less sensitive than PCR, in situ hybridization was useful for localizing the expression of target mRN As with cellular accuracy and with low background staining. In addition, two cases were found to be monoclonal only by in situ hybridization, and not by PCR. The results showed that clonal proliferation is detected with the greatest sensitivity with PCR using small routinely processed biopsy specimens and that a difficulty with the PCR method in terms of cellular localization was partially overcome using a microdissection procedure that provided at least tissue-level accuracy.

 

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