Characterization of the cysteine-rich secretory protein 3 gene as an early-transcribed gene with a putative role in the pathophysiology of Sj�gren's syndrome

Autor:	Haralampos M. Moutsopoulos, George Thyphronitis, Mary Polihronis, Nikolaos I. Tapinos
Rok vydání:	2002
Předmět:	Messenger RNA Differential display Pathology medicine.medical_specialty medicine.diagnostic_test Immunology RNA In situ hybridization Biology Molecular biology Reverse transcription polymerase chain reaction Rheumatology Gene expression Biopsy medicine Immunology and Allergy Pharmacology (medical) Gene
Zdroj:	Arthritis & Rheumatism. 46:215-222
ISSN:	1529-0131 0004-3591
DOI:	10.1002/1529-0131(200201)46:1<215::aid-art10024>3.0.co;2-m
Popis:	Objective To identify genes that may participate in the pathophysiology of Sjogren's syndrome (SS), the technique of differential display was applied to labial minor salivary gland (MSG) biopsy samples. Methods Total RNA was isolated from MSG biopsy samples from a woman with primary SS and a control subject, and the differential display protocol with 8 different random oligonucleotide primers was performed. One particular differentially expressed fragment showed 98% homology with the cysteine-rich secretory protein 3 (CRISP-3) gene. The result was verified by reverse transcription-polymerase chain reaction (RT-PCR) with messenger RNA (mRNA) samples from MSG biopsy tissues obtained from 4 women with primary SS. A CRISP-3 RNA probe was synthesized for in situ hybridization of 7 MSG biopsy samples from patients with primary SS. In an attempt to interpret the expression of CRISP-3, normal peripheral blood lymphocytes (PBLs) were activated in vitro at different time points and assayed for CRISP-3 expression. Finally, B cells were transfected with the coding region of CRISP-3 and monitored for the up-regulation of different B cell activation markers. Results The CRISP-3 gene was detected by RT-PCR in all SS patients tested. Mainly the mononuclear cells infiltrating the MSGs of patients expressed CRISP-3 mRNA. In addition, CRISP-3 was detected by RT-PCR between 30 minutes and 6 hours in phorbol myristate acetate-activated normal PBLs, while staurosporine inhibited this expression. CRISP-3-transfected B cells exhibited an up-regulation in CD25 surface expression. Conclusion The CRISP-3 gene is identified as a novel early response gene that may participate in the pathophysiology of the autoimmune lesions of SS.
Databáze:	OpenAIRE
Externí odkaz:	https://explore.openaire.eu/search/publication?articleId=doi_________::ac7296cc618af2926f59efcd0e5761cf https://doi.org/10.1002/1529-0131(200201)46:1<215::aid-art10024>3.0.co Zobrazit plný text záznamu Plný text