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氨基丙烷羟基二膦酸盐与心包生物假体组织中戊二醛残基的共价结合:稳定性和钙化抑制研究

Covalent binding of aminopropanehydroxydiphosphonate to glutaraldehyde residues in pericardial bioprosthetic tissue: stability and calcification inhibition studies.

作者信息

Webb C L, Schoen F J, Levy R J

机构信息

Section of Pediatric Cardiology, University of Michigan Medical Center, Ann Arbor 48109-0576.

出版信息

Exp Mol Pathol. 1989 Jun;50(3):291-302. doi: 10.1016/0014-4800(89)90039-7.

Abstract

Calcification has limited the clinical utility of bioprosthetic heart valves fabricated from either glutaraldehyde-pretreated bovine pericardium or porcine aortic valves. Aminopropanehydroxydiphosphonate (APDP), covalently bound to residual aldehyde groups in glutaraldehyde-treated pericardial bioprosthetic tissue, has been shown to inhibit cardiovascular calcification in the rat subdermal model. Using 3H-labeled glutaraldehyde (GLUT) at a concentration of 0.02 M and 0.14 M 14C-labeled APDP, we assessed the effects of GLUT incubation temperature (4 degrees or 25 degrees C) and pH of the GLUT incubation solution (pH 4.0, 7.4, or 10.0) on the GLUT incorporation step and subsequent APDP binding (24 hr 25 degrees C) into bioprosthetic valve (BPV) tissue (bovine pericardium). Increased incorporation of GLUT and APDP occurred at lower GLUT incubation temperature (GLUT, 346.05 +/- 1.9 nM/mg, 4 degrees C vs 259.76 +/- 1.39 nM/mg, 25 degrees C; APDP, 57.56 +/- 4.43 nM/mg, 4 degrees C vs 36.36 +/- 0.46 nM/mg, mean +/- standard error, at 25 degrees C). There also was a greater incorporation of GLUT but not APDP at the higher glutaraldehyde pretreatment pH (GLUT, pH 10.0, 213.73 +/- 73 nM/mg vs pH 4, 132.08 +/- 43 nM/mg; APDP, pH 10.0, 51.41 +/- 12 nM/mg vs pH 4.0, 49.97 +/- 6 nM/mg). In vivo studies revealed that all groups with treated BPV implanted for 21 days in male 3-week-old CD rats demonstrated a loss of both GLUT (12-50%) and APDP (48-64%) compared to preimplant content. BPV implant calcification was significantly inhibited in all groups treated with APDP compared to control Ca2+ (5.54 +/- 2.1-9.64 + 1.2 micrograms/mg, APDP pretreated, vs 93.64 +/- 11.65 micrograms/mg, control; P less than or equal to 0.001) despite the progressive loss of both GLUT and APDP with time. It is concluded that preincubation of BPV tissue in GLUT at lower temperature (4 degrees C) and higher pH (10.0) enhanced BPV GLUT uptake and subsequent APDP covalent binding. In addition, in the rat subdermal model, BPV tissue calcification was markedly inhibited by APDP, despite a significant loss of bound drug.

摘要

钙化限制了由戊二醛预处理的牛心包或猪主动脉瓣制成的生物人工心脏瓣膜的临床应用。已证明,与戊二醛处理的心包生物人工组织中的残留醛基共价结合的氨丙基羟基二膦酸盐(APDP)在大鼠皮下模型中可抑制心血管钙化。我们使用浓度为0.02 M的3H标记戊二醛(GLUT)和0.14 M的14C标记APDP,评估了GLUT孵育温度(4℃或25℃)以及GLUT孵育溶液的pH值(pH 4.0、7.4或10.0)对GLUT掺入步骤以及随后APDP在25℃下24小时与生物人工瓣膜(BPV)组织(牛心包)结合的影响。较低的GLUT孵育温度下GLUT和APDP的掺入增加(GLUT,4℃时为346.05±1.9 nM/mg,25℃时为259.76±1.39 nM/mg;APDP,4℃时为57.56±4.43 nM/mg,25℃时为36.36±0.46 nM/mg,均值±标准误)。在较高的戊二醛预处理pH值下GLUT的掺入也更多,但APDP没有(GLUT,pH 10.0时为213.73±73 nM/mg,pH 4时为132.08±43 nM/mg;APDP,pH 10.0时为51.41±12 nM/mg,pH 4.0时为49.97±6 nM/mg)。体内研究显示,在3周龄雄性CD大鼠中植入经处理的BPV 21天的所有组,与植入前含量相比,GLUT(12 - 50%)和APDP(48 - 64%)均有损失。与对照Ca2+相比,所有用APDP处理的组中BPV植入物钙化均受到显著抑制(5.54±2.1 - 9.64 + 1.2微克/毫克,APDP预处理组,对照为93.64±11.65微克/毫克;P≤0.001),尽管随着时间推移GLUT和APDP都逐渐损失。结论是,BPV组织在较低温度(4℃)和较高pH值(10.0)下用GLUT预孵育可增强BPV对GLUT的摄取以及随后APDP的共价结合。此外,在大鼠皮下模型中,尽管结合药物有显著损失,但APDP可显著抑制BPV组织钙化。

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