Translations:High-density lipoprotein/19/ja: Difference between revisions

== Estimating HDL via associated cholesterol ==
Clinical laboratories formerly measured HDL cholesterol by separating other lipoprotein fractions using either ultracentrifugation or chemical precipitation with divalent ions such as Mg²⁺, then coupling the products of a cholesterol oxidase reaction to an indicator reaction. The reference method still uses a combination of these techniques. Most laboratories now use automated homogeneous analytical methods in which lipoproteins containing [[Apolipoprotein B|apo B]] are blocked using antibodies to apo B, then a [[Colorimetry (chemical method)|colorimetric]] enzyme reaction measures cholesterol in the non-blocked HDL particles. [[High-performance liquid chromatography|HPLC]] can also be used. Subfractions (HDL-2C, HDL-3C) can be measured, but clinical significance of these subfractions has not been determined. The measurement of apo-A reactive capacity can be used to measure HDL cholesterol but is thought to be less accurate.