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有证据表明,人红细胞对三碘-L-甲状腺原氨酸的摄取是由载体介导的,但不依赖能量。

Evidence that the uptake of tri-iodo-L-thyronine by human erythrocytes is carrier-mediated but not energy-dependent.

作者信息

Docter R, Krenning E P, Bos G, Fekkes D F, Hennemann G

出版信息

Biochem J. 1982 Oct 15;208(1):27-34. doi: 10.1042/bj2080027.

Abstract

We investigated 3,3',5-tri-iodo-l-thyronine transport by human erythrocytes and by ;ghosts' prepared from these cells. Uptake of tri-iodothyronine by erythrocytes at 37 degrees C was time-dependent with a maximum reached after 60min. Tracer analysis after incubation for 1min revealed only one saturable binding site, with K(m) 128+/-19nm (mean+/-s.e.m.; n=7) and V(max.) 4.6+/-0.7pmol of tri-iodothyronine/min per 6x10(7) cells. After 10min incubation K(m) 100+/-16nm (n=10) was found with V(max.) 7.7+/-1.2pmol of tri-iodothyronine/10min per 6x10(7) cells. At 0 degrees C the uptake system is still active, with K(m) 132+/-26nm and V(max.) 1.8+/-0.3pmol of tri-iodothyronine/10min per 6x10(7) cells. The V(max.) with intact cells is 5-fold greater than the V(max.) with membranes derived from the same amount of cells when uptake studies are performed in media with similar free tri-iodothyronine concentrations. This indicates that at least 80% of tri-iodothyronine taken up by the intact erythrocytes enters the cell. This saturable uptake system can be inhibited by X-ray-contrast agents in a dose-dependent fashion. (+/-)-Propranolol, but not atenolol, has the same effect, indicating that the membrane-stabilizing properties of (+/-)-propranolol are involved. Furthermore, there is no inhibition by ouabain or vanadate, which indicates that tri-iodothyronine uptake is not dependent on the activity of Na(+)+K(+)-dependent adenosine triphosphatase. We have prepared erythrocyte ;ghosts', resealed after 2.5min with 0mm-, 2mm- or 4mm-ATP inside. Inclusion of ATP and integrity of the membrane of the erythrocyte ;ghosts' were verified on the basis of an ATP-concentration-dependent functioning of the Ca(2+) pump. No difference was found in the uptake of tri-iodothyronine by erythrocyte ;ghosts' with or without ATP included, indicating that uptake of tri-iodothyronine is not ATP-dependent. The following conclusions are drawn. (1) Tri-iodothyronine enters human erythrocytes. (2) There is only one saturable uptake system present for tri-iodothyronine, which is neither energy (i.e. ATP)-dependent nor influenced by the absence of an Na(+) gradient across the plasma membrane. This mode of uptake of tri-iodothyronine by human erythrocytes is in sharp contrast with that of rat hepatocytes, which uptake system is energy-dependent and ouabain-sensitive [Krenning, Docter, Bernard, Visser & Hennemann (1978) FEBS Lett.91, 113-116; Krenning, Docter, Bernard, Visser & Hennemann (1980) FEBS Lett.119, 279-282]. (3) X-ray-contrast agents inhibit tri-iodothyronine uptake by erythrocytes in a similar fashion to that by which they inhibit the uptake of tri-iodothyronine by rat hepatocytes [Krenning, Docter, Bernard, Visser & Hennemann (1982) FEBS Lett.140, 229-233].

摘要

我们研究了人红细胞及由这些细胞制备的“血影”对3,3',5-三碘-L-甲状腺原氨酸的转运。红细胞在37℃对三碘甲状腺原氨酸的摄取呈时间依赖性,60分钟后达到最大值。孵育1分钟后的示踪分析显示只有一个可饱和结合位点,米氏常数(K(m))为128±19nM(平均值±标准误;n = 7),最大转运速率(V(max.))为每6×10(7)个细胞每分钟摄取4.6±0.7pmol三碘甲状腺原氨酸。孵育10分钟后,K(m)为100±16nM(n = 10),V(max.)为每6×10(7)个细胞每10分钟摄取7.7±1.2pmol三碘甲状腺原氨酸。在0℃时摄取系统仍有活性,K(m)为132±26nM,V(max.)为每6×10(7)个细胞每10分钟摄取1.8±0.3pmol三碘甲状腺原氨酸。当在具有相似游离三碘甲状腺原氨酸浓度的培养基中进行摄取研究时,完整细胞的V(max.)比由相同数量细胞衍生的膜的V(max.)大5倍。这表明完整红细胞摄取的三碘甲状腺原氨酸中至少80%进入细胞。这种可饱和摄取系统可被X射线造影剂以剂量依赖性方式抑制。(±)-普萘洛尔而非阿替洛尔有相同作用,表明涉及(±)-普萘洛尔的膜稳定特性。此外,哇巴因或钒酸盐无抑制作用,这表明三碘甲状腺原氨酸摄取不依赖于Na(+)+K(+)-依赖性腺苷三磷酸酶的活性。我们制备了红细胞“血影”,在2.5分钟后用细胞内0mM、2mM或4mM的ATP重新封闭。根据Ca(2+)泵的ATP浓度依赖性功能验证了ATP的存在及红细胞“血影”膜的完整性。有无ATP的红细胞“血影”对三碘甲状腺原氨酸的摄取未发现差异,表明三碘甲状腺原氨酸摄取不依赖于ATP。得出以下结论。(1)三碘甲状腺原氨酸进入人红细胞。(2)三碘甲状腺原氨酸只有一个可饱和摄取系统,该系统既不依赖能量(即ATP),也不受跨质膜Na(+)梯度缺失的影响。人红细胞摄取三碘甲状腺原氨酸的这种方式与大鼠肝细胞形成鲜明对比,大鼠肝细胞的摄取系统依赖能量且对哇巴因敏感[克伦宁、多克特、伯纳德、维瑟和亨内曼(1978年)《欧洲生物化学学会联合会快报》91,113 - 116;克伦宁、多克特、伯纳德、维瑟和亨内曼(1980年)《欧洲生物化学学会联合会快报》119,279 - 282]。(3)X射线造影剂抑制红细胞摄取三碘甲状腺原氨酸的方式与抑制大鼠肝细胞摄取三碘甲状腺原氨酸的方式相似[克伦宁、多克特、伯纳德、维瑟和亨内曼(1982年)《欧洲生物化学学会联合会快报》140,229 - 233]。

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