Department of Physiology and Biophysics, Boston University School of Medicine, Boston, Massachusetts 02118, United States.
Biochemistry. 2012 Feb 14;51(6):1238-48. doi: 10.1021/bi2015212. Epub 2012 Feb 2.
Apolipoprotein C-I (apoC-I) is an important constituent of high-density lipoprotein (HDL) and is involved in the accumulation of cholesterol ester in nascent HDL via inhibition of cholesterol ester transfer protein and potential activation of lecithin:cholesterol acyltransferase (LCAT). As the smallest exchangeable apolipoprotein (57 residues), apoC-I transfers between lipoproteins via a lipid-binding motif of two amphipathic α-helices (AαHs), spanning residues 7-29 and 38-52. To understand apoC-I's behavior at hydrophobic lipoprotein surfaces, oil drop tensiometry was used to compare the binding to triolein/water (TO/W) and palmitoyloleoylphosphatidylcholine/triolein/water (POPC/TO/W) interfaces. When apoC-I binds to either interface, the surface tension (γ) decreases by ~16-18 mN/m. ApoC-I can be exchanged at both interfaces, desorbing upon compression and readsorbing on expansion. The maximal surface pressures at which apoC-I begins to desorb (Π(max)) were 16.8 and 20.7 mN/m at TO/W and POPC/TO/W interfaces, respectively. This suggests that apoC-I interacts with POPC to increase its affinity for the interface. ApoC-I is more elastic on POPC/TO/W than TO/W interfaces, marked by higher values of the elasticity modulus (ε) on oscillations. At POPC/TO/W interfaces containing an increasing POPC:TO ratio, the pressure at which apoC-I begins to be ejected increases as the phospholipid surface concentration increases. The observed increase in apoC-I interface affinity due to higher degrees of apoC-I-POPC interactions may explain how apoC-I can displace larger apolipoproteins, such as apoE, from lipoproteins. These interactions allow apoC-I to remain bound to the interface at higher Π values, offering insight into apoC-I's rearrangement on triacylglycerol-rich lipoproteins as they undergo Π changes during lipoprotein maturation by plasma factors such as lipoprotein lipase.
载脂蛋白 C-I (apoC-I) 是高密度脂蛋白 (HDL) 的重要组成部分,通过抑制胆固醇酯转移蛋白并可能激活卵磷脂:胆固醇酰基转移酶 (LCAT),参与新生 HDL 中胆固醇酯的积累。作为最小的可交换载脂蛋白 (57 个残基),apoC-I 通过两个两亲性α-螺旋 (AαHs) 的脂质结合基序在脂蛋白之间转移,跨越残基 7-29 和 38-52。为了了解 apoC-I 在疏水性脂蛋白表面的行为,使用油滴张力计比较了与三油酸甘油酯/水 (TO/W) 和棕榈酰油酰基卵磷脂/三油酸甘油酯/水 (POPC/TO/W) 界面的结合。当 apoC-I 结合到任一界面时,表面张力 (γ) 降低约 16-18 mN/m。apoC-I 可以在两个界面上交换,在压缩时解吸,在膨胀时重新吸附。apoC-I 开始解吸的最大表面压力 (Π(max)) 在 TO/W 和 POPC/TO/W 界面分别为 16.8 和 20.7 mN/m。这表明 apoC-I 与 POPC 相互作用以增加其与界面的亲和力。apoC-I 在 POPC/TO/W 上比在 TO/W 界面上更具弹性,这表现为在振荡时弹性模量 (ε) 的值更高。在含有逐渐增加的 POPC:TO 比例的 POPC/TO/W 界面上,随着磷脂表面浓度的增加,apoC-I 开始被弹出的压力增加。apoC-I 与 POPC 相互作用程度增加导致 apoC-I 界面亲和力增加,这可能解释了 apoC-I 如何从脂蛋白中置换更大的载脂蛋白,如 apoE。这些相互作用使 apoC-I 能够在更高的 Π 值下保持与界面结合,为 apoC-I 在富含三酰基甘油的脂蛋白上的重排提供了深入的了解,因为它们在脂蛋白成熟过程中会经历 Π 变化,这是由脂蛋白脂肪酶等血浆因子引起的。
