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内因子介导的豚鼠回肠细胞对钴胺素的吸收。

Intrinsic factor-mediated absorption of cobalamin by guinea pig ileal cells.

作者信息

Kapadia C R, Serfilippi D, Voloshin K, Donaldson R M

出版信息

J Clin Invest. 1983 Mar;71(3):440-8. doi: 10.1172/jci110788.

Abstract

To investigate the fate of intrinsic factor and cobalamin during cobalamin absorption, we incubated enterocytes isolated from guinea pig ileum for periods of up to 30 min with (57)Co-labeled cyano-cobalamin bound either to human intrinsic factor or to rabbit intrinsic factor biosynthetically labeled with [(35)S]methionine. When the labeled complex was incubated for 30 min with isolated ileal cells under conditions that block cellular metabolism, virtually all cellular radioactivity could be removed by washing the cell surface with EDTA or acid. In contrast, washing removed only half the radioactivity from cells incubated at 37 degrees C in O(2). When residual cellular radioactivity was extracted and analyzed by gel filtration, 80-94% of both the (35)S and (57)Co radioactivity eluted in the same fractions as the original complex. The remaining 6-20% eluted as free [(57)Co]cobalamin or [(35)S]methionine. To examine events occurring after 30 min, we instilled into tied-off ileal loops of intact guinea pigs radiolabeled intrinsic factor-cobalamin complex and extracted nondissociable radioactivity 2-4.5 h later. The proportion of extracted (57)Co eluting as free cobalamin increased to 39-46%, that eluting as intrinsic factor-cobalamin complex declined to 22-45%, and 9-34% now eluted as a macromolecule that reacted with antitranscobalamin II antibody but not antiintrinsic factor antibody. Extracted (35)S radioactivity eluted in several peaks in addition to the intrinsic factor peak. These findings suggest that (a) after reversible attachment of intrinsic factor-cobalamin complex to its ileal surface receptor, an energy-dependent process prevents removal of the complex from the cell surface by EDTA or acid; (b) cobalamin dissociates from intrinsic factor and, as suggested by previous workers, binds to a molecule antigenically similar to transcobalamin II; and (c) intrinsic factor is slowly degraded and forms breakdown products that are detectable in ileal extracts.

摘要

为研究钴胺素吸收过程中内因子和钴胺素的命运,我们将从豚鼠回肠分离的肠上皮细胞与结合了人内因子或用[³⁵S]甲硫氨酸生物标记的兔内因子的(⁵⁷)Co标记的氰钴胺一起孵育长达30分钟。当标记复合物在阻断细胞代谢的条件下与分离的回肠细胞孵育30分钟时,几乎所有细胞放射性都可通过用EDTA或酸洗涤细胞表面而去除。相比之下,洗涤只能从在37℃于O₂中孵育的细胞中去除一半放射性。当提取残留的细胞放射性并通过凝胶过滤分析时,80 - 94%的³⁵S和⁵⁷Co放射性与原始复合物在相同组分中洗脱。其余6 - 20%以游离的[⁵⁷Co]钴胺素或[³⁵S]甲硫氨酸形式洗脱。为检查30分钟后发生的事件,我们将放射性标记的内因子 - 钴胺素复合物注入完整豚鼠的结扎回肠袢中,并在2 - 4.5小时后提取不可解离的放射性。以游离钴胺素形式洗脱的提取的⁵⁷Co比例增加到39 - 46%,以内因子 - 钴胺素复合物形式洗脱的比例降至22 - 45%,现在有9 - 34%以与抗转钴胺素II抗体反应但不与抗内因子抗体反应的大分子形式洗脱。提取的³⁵S放射性除了内因子峰外还在几个峰中洗脱。这些发现表明:(a)内因子 - 钴胺素复合物可逆地附着于其回肠表面受体后,一个能量依赖过程可防止该复合物被EDTA或酸从细胞表面去除;(b)钴胺素从内因子解离,并且如先前研究者所提示的,与一种抗原性类似于转钴胺素II的分子结合;(c)内因子被缓慢降解并形成在回肠提取物中可检测到的分解产物。

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