Abstract

A variety of methods are currently used to analyze HL and LPL activities in mice. In search of a simple methodology, we analyzed mouse preheparin and postheparin plasma LPL and HL activities using specific polyclonal antibodies raised in rabbit against rat HL (anti-HL) and in goat against rat LPL (anti-LPL). As an alternative, we analyzed HL activity in the presence of 1 M NaCl, a condition known to inhibit LPL activity in humans. The assays were validated using plasma samples from wild-type and HL-deficient C57BL/6 mice. We now show that the use of 1 M NaCl for the inhibition of plasma LPL activity in mice may generate incorrect measurements of both LPL and HL activities. Our data indicate that HL can be measured directly, without heparin injection, in preheparin plasma, because virtually all HL is present in an unbound form circulating in plasma. In contrast, measurable LPL activity is present only in postheparin plasma. Both HL and LPL can be measured using the same assay conditions (low salt and the presence of apolipoprotein C-II as an LPL activator). Total lipase activity in postheparin plasma minus preheparin HL activity reflects LPL activity. Specific antibodies are not required.

Highlights

  • A variety of methods are currently used to analyze HL and LPL activities in mice

  • It is generally accepted that lipase activity in murine preheparin plasma represents HL activity [3], reflecting its low affinity for heparin sulfate proteoglycans

  • Zero lipase activity was measured in preheparin plasma from HL-deficient mice

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Summary

Appraisal of hepatic lipase and lipoprotein lipase activities in mice

C. van Vark-van der Zee,§ R. van Haperen,** T. van Gent,** H.

MATERIALS AND METHODS
Treatment of plasma with antibodies
Lipase assay
RESULTS AND DISCUSSION
Full Text
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