Inhibition and promotion of cholesterol crystallization by protein fractions from normal human gallbladder bile

Inhibition and promotion of cholesterol crystallization by protein fractions from normal human gallbladder bile

Pooled, normal human gallbladder biles were initially separated on a molecular sieving chromatography column to remove soluble mucin glycoproteins as well as high molecular weight proteins (greater than 200,000). The remaining lower molecular weight proteins and other bile components were then exami...

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Main Authors: N Busch, N Matiuck, S Sahlin, SP Pillay, RT Holzbach
Format: Article
Language:English
Published: Elsevier 1991-04-01
Series:Journal of Lipid Research
Online Access:http://www.sciencedirect.com/science/article/pii/S0022227520420577
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spelling doaj-f6cf0650510e4b13a9b02018c0204cec2021-04-25T04:21:35ZengElsevierJournal of Lipid Research0022-22751991-04-01324695702Inhibition and promotion of cholesterol crystallization by protein fractions from normal human gallbladder bileN Busch0N Matiuck1S Sahlin2SP Pillay3RT Holzbach4Department of Gastroenterology, Cleveland Clinic Foundation, OH 44195-5218.Department of Gastroenterology, Cleveland Clinic Foundation, OH 44195-5218.Department of Gastroenterology, Cleveland Clinic Foundation, OH 44195-5218.Department of Gastroenterology, Cleveland Clinic Foundation, OH 44195-5218.Department of Gastroenterology, Cleveland Clinic Foundation, OH 44195-5218.Pooled, normal human gallbladder biles were initially separated on a molecular sieving chromatography column to remove soluble mucin glycoproteins as well as high molecular weight proteins (greater than 200,000). The remaining lower molecular weight proteins and other bile components were then examined by lectin affinity chromatography with four different types of lectin. The separated bound fractions were compared for inhibiting and promoting activities with a newly devised sensitive cholesterol crystal growth assay and for differences in electrophoretic patterns on SDS-gels. Protein factors (presumably glycoproteins) were found to have both inhibiting and promoting activities, even in the absence of cholesterol gallstone disease. The promoting effect was indicated by shortened crystal detection times and increases in crystal growth rate; whereas the inhibiting effect was indicated by decreases in crystal growth rate and reductions in the final crystal concentration as determined by the growth assay. Affinity chromatography mitigated the major problems of removing both lipids and pigment from the glycoproteins. In addition, partial purification of bound fractions with potent cholesterol crystal nucleation-altering activity can be obtained by this technique.http://www.sciencedirect.com/science/article/pii/S0022227520420577
collection DOAJ
language English
format Article
sources DOAJ
author N Busch
N Matiuck
S Sahlin
SP Pillay
RT Holzbach
spellingShingle N Busch
N Matiuck
S Sahlin
SP Pillay
RT Holzbach
Inhibition and promotion of cholesterol crystallization by protein fractions from normal human gallbladder bile
Journal of Lipid Research
author_facet N Busch
N Matiuck
S Sahlin
SP Pillay
RT Holzbach
author_sort N Busch
title Inhibition and promotion of cholesterol crystallization by protein fractions from normal human gallbladder bile
title_short Inhibition and promotion of cholesterol crystallization by protein fractions from normal human gallbladder bile
title_full Inhibition and promotion of cholesterol crystallization by protein fractions from normal human gallbladder bile
title_fullStr Inhibition and promotion of cholesterol crystallization by protein fractions from normal human gallbladder bile
title_full_unstemmed Inhibition and promotion of cholesterol crystallization by protein fractions from normal human gallbladder bile
title_sort inhibition and promotion of cholesterol crystallization by protein fractions from normal human gallbladder bile
publisher Elsevier
series Journal of Lipid Research
issn 0022-2275
publishDate 1991-04-01
description Pooled, normal human gallbladder biles were initially separated on a molecular sieving chromatography column to remove soluble mucin glycoproteins as well as high molecular weight proteins (greater than 200,000). The remaining lower molecular weight proteins and other bile components were then examined by lectin affinity chromatography with four different types of lectin. The separated bound fractions were compared for inhibiting and promoting activities with a newly devised sensitive cholesterol crystal growth assay and for differences in electrophoretic patterns on SDS-gels. Protein factors (presumably glycoproteins) were found to have both inhibiting and promoting activities, even in the absence of cholesterol gallstone disease. The promoting effect was indicated by shortened crystal detection times and increases in crystal growth rate; whereas the inhibiting effect was indicated by decreases in crystal growth rate and reductions in the final crystal concentration as determined by the growth assay. Affinity chromatography mitigated the major problems of removing both lipids and pigment from the glycoproteins. In addition, partial purification of bound fractions with potent cholesterol crystal nucleation-altering activity can be obtained by this technique.
url http://www.sciencedirect.com/science/article/pii/S0022227520420577
work_keys_str_mv AT nbusch inhibitionandpromotionofcholesterolcrystallizationbyproteinfractionsfromnormalhumangallbladderbile
AT nmatiuck inhibitionandpromotionofcholesterolcrystallizationbyproteinfractionsfromnormalhumangallbladderbile
AT ssahlin inhibitionandpromotionofcholesterolcrystallizationbyproteinfractionsfromnormalhumangallbladderbile
AT sppillay inhibitionandpromotionofcholesterolcrystallizationbyproteinfractionsfromnormalhumangallbladderbile
AT rtholzbach inhibitionandpromotionofcholesterolcrystallizationbyproteinfractionsfromnormalhumangallbladderbile
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