1990
DOI: 10.1111/j.1432-1033.1990.tb15587.x
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Molecular characterization of three rat liver serine‐protease inhibitors affected by inflammation and hypophysectomy

Abstract: Rat hepatocytes have the potential to secrete three similar acidic glycoproteins, serine protease inhibitors 1, 2 and 3 (SPI-1, SPI-2, SPI-3), recognized by the same antibodies. They were synthesized as precursors of comparable sizes (45 kDa), which were post-translationally modified by N-glycosylation at three (SPI-3) or four (SPI-1 and SPI-2) sites. This appeared to account for the size difference of mature proteins. The mRNA sequences, derived from cDNA clones, displayed a high degree of similarity (70-90%)… Show more

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Cited by 53 publications
(43 citation statements)
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“…It has been shown that inflammation causes a decrease in the Spi 2 expression. 26 AdCTGF and AdTGF␤1 up-regulate Spi 2 RNA in mouse liver compared with the adenoviral control AdE1. Spi 2 is constitutively expressed in liver tissue of normal rats and significantly decreased during inflammation.…”
Section: Discussionmentioning
confidence: 92%
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“…It has been shown that inflammation causes a decrease in the Spi 2 expression. 26 AdCTGF and AdTGF␤1 up-regulate Spi 2 RNA in mouse liver compared with the adenoviral control AdE1. Spi 2 is constitutively expressed in liver tissue of normal rats and significantly decreased during inflammation.…”
Section: Discussionmentioning
confidence: 92%
“…Spi 2 is constitutively expressed in liver tissue of normal rats and significantly decreased during inflammation. 26 The up-regulation of protease inhibitors is a common feature of overexpression of TGF␤1 and CTGF and may reflect the role that these genes play in fibrosis. 6,18 It has been shown that synthetic serine protease inhibitors, in combination with a metalloprotease 1 inhibitor, prevent the invasion and metastasis of tumor cells 27 by inhibiting the degradation of the extra-cellular matrix.…”
Section: Discussionmentioning
confidence: 99%
“…The procedure for run-on analysis, which includes incubation of the nuclei with [a-"PIUTP, purification of total cellular RNA and hybridization to templates immobilized on a nylon membrane (Hybond NC, Amersham) has been previously described [16]. The following plasmids were used as hybridization templates: pUC19 bearing 0.52 kb of the spi 2.1 cDNA 5' region [2]; pUC19 bearing the 0.35-kb 3' UTR specific extension of the spi 2.3 gene [2]; pBR322 harboring 0.65 kb of the rat a,-macroglobulin cDNA [17]; pBR322 bearing 1.6 kb of the mouse p-actin cDNA [18]; pBR322 containing 1.2 kb of the rat albumin cDNA [19]; Bluescript SK+ bearing 0.7 kb of the rat a,-acid glycoprotein cDNA [20]; pUC 19 bearing 1.25 kb of the rat insulin receptor tyrosine kinase inhibitor cDNA @p63) [21]. The amount of labeled transcripts newly synthetized by control and inflamed rat liver nuclei used for hybridization to templates corresponded to 20 X 1 O6 trichloroacetic-acid-precipitable counts.…”
Section: Materials [A-32p]datp (3000 Cdmmolmentioning
confidence: 99%
“…Nuclei isolated from the liver [15] of normal or turpentine inflamed rats [2] were used to evaluate the in vivo rates of transcription initiation. The procedure for run-on analysis, which includes incubation of the nuclei with [a-"PIUTP, purification of total cellular RNA and hybridization to templates immobilized on a nylon membrane (Hybond NC, Amersham) has been previously described [16].…”
Section: Materials [A-32p]datp (3000 Cdmmolmentioning
confidence: 99%
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