Lipoprotein Lipase: Some Effects of Activator Proteins
- 1 May 1980
- journal article
- research article
- Published by Wiley in European Journal of Biochemistry
- Vol. 106 (2) , 549-555
- https://doi.org/10.1111/j.1432-1033.1980.tb04602.x
Abstract
The stimulation by apolipoprotein CII from human plasma lipoproteins and T1 and T2 proteins from egg yolk lipoproteins of the activity of [bovine milk] lipoprotein lipase was studied. These activator proteins stabilized the enzyme much more effectively than a 1000-fold higher concentration of albumin did, indicating direct interaction with the enzyme. The effects of the activators were seen also at 1 M NaCl. Forces other than electrostatic are implicated. Centrifugation experiments showed that 125I-labeled lipase bound equally well to the emulsion droplets in the absence of activator protein as in its presence. This was true even under conditions when the activator caused a severalfold increase in the rate of hydrolysis. The activator makes enzyme at the interface more effective in hydrolysis. By optimizing the conditions it was possible to obtain almost as high rates of triglyceride hydrolysis in the absence as in the presence of activator. The main effect of the activator protein is probably not on a rate-limiting chemical step. Under most condition, the rate of hydrolysis was much below optimal, and activator increased it. This was always the case with phosphatidylcholine/triglyceride emulsions, where the activator enhanced hydrolysis of both lipids. Other experiments showed that the activator enhanced triglyceride hydrolysis in the absence of phospholipids and phospholipid hydrolysis in the absence of triglycerides. Interaction with activator orientates the enzyme and/or the lipid substrate for effective hydrolysis at the surface of lipoproteins/model substrates.This publication has 38 references indexed in Scilit:
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