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在β6位置带有碱性氨基酸取代(赖氨酸和精氨酸)的重组血红蛋白的结晶。

Crystallization of recombinant hemoglobins with basic amino acid substitutions (Lys and Arg) at the beta 6 position.

作者信息

Adachi K, Lai C H, Konitzer P, Donahee M, Campbell A, Surrey S

机构信息

Division of Hematology, Children's Hospital of Philadelphia, PA 19104.

出版信息

Blood. 1994 Aug 15;84(4):1309-13.

PMID:8049445
Abstract

We have produced recombinant hemoglobins (rHbs) alpha 2 beta 2(6Glu-->Lys) (rHb beta E6K) and alpha 2 beta 2(6Glu-->Arg) (rHb beta E6R) using a yeast expression system coupled with a polymerase chain reaction (PCR)-based mutagenesis strategy for studies focused on defining determinants that facilitate crystallization of Hb C (alpha 2 beta 2(6Lys)). rHb beta E6K had the same electrophoretic mobility as native human Hb C, whereas rHb beta E6R migrated slightly slower than Hb C on cellulose acetate electrophoresis. The carbonmonoxy (CO) forms of rHb beta E6K and rHb beta E6R formed tetrahedral crystals in vitro in 2.3 mol/L phosphate buffer just like native Hb C. The Hb concentration required for crystallization of CO-rHb beta E6R was lower than that of CO-rHb beta E6K, suggesting that stronger basic amino acids at the beta 6 position accelerate crystallization of Hb. However, the size of rHb beta E6R crystals was smaller than that of rHb beta E6K. Crystallization of native Hb C and both rHbs was inhibited by Hb F. These results suggest that alpha 2 beta gamma-heterohybrids that have basic amino acids at the beta 6 position behave similarly and are unable to crystallize like Hb C.

摘要

我们利用酵母表达系统结合基于聚合酶链反应(PCR)的诱变策略,制备了重组血红蛋白(rHbs)α2β2(6Glu→Lys)(rHb βE6K)和α2β2(6Glu→Arg)(rHb βE6R),用于聚焦于确定促进Hb C(α2β2(6Lys))结晶的决定因素的研究。rHb βE6K在电泳迁移率上与天然人Hb C相同,而rHb βE6R在醋酸纤维素电泳上的迁移速度略慢于Hb C。rHb βE6K和rHb βE6R的一氧化碳(CO)形式在体外2.3 mol/L磷酸盐缓冲液中形成四面体晶体,就像天然Hb C一样。CO-rHb βE6R结晶所需的血红蛋白浓度低于CO-rHb βE6K,这表明β6位更强的碱性氨基酸加速了血红蛋白的结晶。然而,rHb βE6R晶体的尺寸小于rHb βE6K。天然Hb C和两种rHbs的结晶均受到Hb F的抑制。这些结果表明,在β6位具有碱性氨基酸的α2βγ-异源杂种表现相似,且不能像Hb C那样结晶。

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