Wavelength Selection in Hemolytic Evaluation Systems with Spectrophotometry Detection_Journal of Biomedical Engineering

Authors：

ZHANGHong ¹ , SUBaochang ² , YEXunda ¹ ,  LUOMan ¹

1. College of Life Science and Technology, Jinan University, Guangzhou 510632, China;
2. Department of Blood Transfusion, The First Affiliated Hospital of Jinan University, Guangzhou 510630, China;

Corresponding author：

LUOMan, Email: txionglu@jnu.edu.cn

Keywords：

hemolytic evaluation; spectrophotometry; red blood cells; hemoglobin; banked blood

DOI：

10.7507/1001-5515.20160062

Video：

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Spectrophotometry is a simple hemolytic evaluation method commonly used in new drugs, biomedical materials and blood products. It is for the quantitative analysis of the characteristic absorption peaks of hemoglobin. Therefore, it is essential to select the correct detection wavelength when the evaluation system has influences on the conformation of hemoglobin. Based on the study of changes in the characteristic peaks over time of the hemolysis supernatant in four systems, namely, cell culture medium, phosphate buffered saline (PBS), physiological saline and banked blood preservation solution, using continuous wavelength scanning, the selections of detection wavelength were proposed as follows. In the cell culture medium system, the wavelength of 415 nm should be selected within 4 h; , near 408 nm should be selected within 4~72 h. In PBS system, within 4 h, 541 nm, 577 nm or 415 nm should be selected; 4~72 h, 541 nm, 577 nm or near 406 nm should be selected. In physiological saline system, within 4 h, 414 nm should be selected; 4~72 h, near 405 nm should be selected; within 12 h, 541 nm or 577 nm could also be selected. In banked blood preservation solution system, within 72 h, 415 nm, 540 nm or 576 nm should be selected.

Citation： ZHANGHong, SUBaochang, YEXunda, LUOMan. Wavelength Selection in Hemolytic Evaluation Systems with Spectrophotometry Detection. Journal of Biomedical Engineering, 2016, 33(2): 368-372. doi: 10.7507/1001-5515.20160062 Copy

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1. 王毅民.血标本溶血的原因及应对措施[J].中国药物与临床, 2013, 13(2):260-261.
2. 胡望平, 胡盈莹, 冯福英, 等.介绍一种测定溶血的高灵敏度方法[J].生物医学工程学杂志, 2007, 24(3):664-666.
3. 中华人民共和国国家质量监督检验检疫总局.GB 18469-2001全血及成分血质量要求[S].中华人民共和国国家标准, 2001:1-14.
4. 掌友湖, 梁启忠, 程玉根.全血质控物配制标准液在血浆游离血红蛋白测定中的应用[J].中国输血杂志, 2009(10):823-824.
5. 周承涛, 卿茂英.溶血试验检测ACD-B血液保养液质量[J].中国输血杂志, 1996, (1):32.
6. 张伶俐, 朱蔚精, 谭言飞, 等.生物材料溶血性标准化评价方法比较:溶血率法和氰化高铁血红蛋白法[J].生物医学工程学杂志, 2004, 21(1):111-114, 137.
7. 张红霞, 刘海侠, 洪庆福, 等.牛血清中牛血红蛋白测定方法的比较及新方法的建立[J].河北医药, 2012, (6):927-928.
8. SOWEMIMO-COKER S O. Red blood cell hemolysis during processing[J]. Transfus Med Rev, 2002, 16(1):46-60.
9. 李娟.卟啉对农药残留的光谱检测及作用关系[D].重庆:重庆大学, 2012.
10. 戴宇飞, 常平, 李桂兰, 等.活性氧对血红蛋白损伤机理的研究[J].卫生研究, 1999, 28(1):30-32.
11. VITELLO L B, ERMAN J E, MILLER M A, et al. Effect of Asp-235.fwdarw.Asn substitution on the absorption spectrum and hydrogen peroxide reactivity of cytochrome c peroxidase[J]. Biochemistry, 1992, 31(46):11524-11535.
12. 张世彪.人类的血红蛋白[J].生物学教学, 1993, (3):1-5.
13. 薛彩福, 郭建明, 钱大玮, 等.黄葵醇提物中黄酮类成分在体肠吸收研究[J].药学学报, 2011, 46(4):454-459.
14. 李平, 刘梅川, 张成林, 等.聚乙烯吡咯烷酮/硫化镉量子点修饰电极的制备及其对血红蛋白的测定研究[J].化学学报, 2005, 63(12):1075-1080, 1032.
15. 秦文斌.血红蛋白的结构与功能——分子呼吸[J].国外医学:分子生物学分册, 1980, (3):109-116.
16. 吴正洁, 康立丽, 黄宝添, 等.pH值对人离体血红蛋白结构及功能的影响[J].生物物理学报, 2009, (S1):334-335.
17. 姚成灿, 黄耀熊.单个活态红细胞血红蛋白随pH值变化的显微分光光度分析[J].中国医学物理学杂志, 2003, 20(4):243-244, 248.
18. 郑素玲.血浆中的血红蛋白为何不能载氧[J].生物学通报, 1999, 34, (7):24.
19. LIU Huihong, TIAN Zhiquan, LU Zhexue, et al. Direct electrochemistry and electrocatalysis of heme-proteins entrapped in agarose hydrogel films[J]. Biosens Bioelectron, 2004, 20(2):294-304.

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