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利用聚(4-氰基联苯-4'-氧基十一烷基丙烯酸酯-b-((2-二甲基氨基)甲基丙烯酸乙酯))功能化的液晶/水界面的生物传感器。

Biosensor utilizing a liquid crystal/water interface functionalized with poly(4-cyanobiphenyl-4'-oxyundecylacrylate-b-((2-dimethyl amino) ethyl methacrylate)).

作者信息

Omer Muhammad, Khan Mashooq, Kim Young Kyoo, Lee Joon Hyung, Kang Inn-Kyu, Park Soo-Young

机构信息

School of Applied Chemical Engineering, Kyungpook National University, Daegu 702-701, Republic of Korea.

School of Advanced Materials Engineering, Kyungpook National University, Daegu 702-701, Republic of Korea.

出版信息

Colloids Surf B Biointerfaces. 2014 Sep 1;121:400-8. doi: 10.1016/j.colsurfb.2014.06.028. Epub 2014 Jun 25.

Abstract

The interface between the nematic liquid crystal, 4-cyano-4'-pentylbiphenyl (5CB) and water within a transmission electron microscopy (TEM) grid cell coated with the pH-dependent weak cationic amphiphilic block copolymer poly((4-cyanobiphenyl-4'-oxyundecylacrylate)-b-((2-dimethyl amino) ethyl methacrylate)) (LCP-b-PDMAEMA) (which was successfully synthesized by reversible addition-fragmentation chain transfer (RAFT) polymerization) was subsequently evaluated for protein and deoxyribonucleic acid (DNA) detection. The LCP-b-PDMAEMA monolayer was fabricated using a Langmuir Blodgett trough, transferred to the 5CB-filled TEM grid, and placed on the octadecyltrichlorosilane-coated glass (TEMPDMAEMA) in such a way that the LCP chains were immersed in the 5CB while the PDMAEMA chains were pointed away from the 5CB surface and immersed in water. Several model proteins such as bovine serum albumin (BSA), hemoglobin (Hb), and chymotrypsinogen (ChTg) were tested at pH values ranging from 2 to 12 to determine the role of the charge state of the protein on protein detection by a weak polyelectrolyte such as PDMAEMA. PDMAEMA contains cationic and neutral states below and above the pKa value, respectively, and is thus able to absorb proteins below its pKa threshold through electrostatic interactions. BSA exhibited a homeotropic to planar (H-P) change in orientation within the TEMPDMAEMA grid cell at concentrations greater than 0.02wt% within the pH range between the isoelectric point (pI) of BSA and the pKa of PDMAEMA, where the charge states of BSA and PDMAEMA were negative and positive, respectively. However, this change in orientation did not occur with other proteins that exhibited a pI higher than the pKa of PDMAEMA due to the electrostatic repulsions resulting from their same cationic charges. This result indicates that the electrostatic interactions between proteins and PDMAEMA are a major contributing factor for protein detection by the H-P transformation within the TEMPDMAEMA grid cell. DNA, a pH-independent strong anionic polyelectrolyte, was also tested with the TEMPDMAEMA grid cell, and it exhibited an H-P transformation at the charged state of PDMAEMA below its pKa threshold at concentrations higher than 0.01wt%. Thus, we demonstrated that the TEMPDMAEMA grid cell effectively facilitated the detection of negatively charged biomaterials (i.e.; protein and DNA) through the H-P transformation using the polarized optical microscope. This simple and inexpensive experimental set-up for non-specific biomaterial detection lays the basic groundwork for developing effective biosensors using polyelectrolytes.

摘要

随后,对涂覆有pH依赖性弱阳离子两亲性嵌段共聚物聚((4-氰基联苯-4'-氧基十一烷基丙烯酸酯)-b-((2-二甲基氨基)甲基丙烯酸乙酯))(LCP-b-PDMAEMA)(通过可逆加成-断裂链转移(RAFT)聚合成功合成)的透射电子显微镜(TEM)网格单元内的向列型液晶4-氰基-4'-戊基联苯(5CB)与水之间的界面进行了蛋白质和脱氧核糖核酸(DNA)检测评估。使用Langmuir Blodgett槽制备LCP-b-PDMAEMA单层,转移到填充有5CB的TEM网格上,并以这样的方式放置在十八烷基三氯硅烷涂覆的玻璃(TEMPDMAEMA)上:LCP链浸入5CB中,而PDMAEMA链远离5CB表面并浸入水中。测试了几种模型蛋白质,如牛血清白蛋白(BSA)、血红蛋白(Hb)和胰凝乳蛋白酶原(ChTg),在pH值范围为2至12,以确定蛋白质的电荷状态对由弱聚电解质如PDMAEMA进行蛋白质检测的作用。PDMAEMA分别在pKa值以下和以上包含阳离子和中性状态,因此能够在其pKa阈值以下通过静电相互作用吸收蛋白质。在BSA的等电点(pI)和PDMAEMA的pKa之间的pH范围内,当BSA浓度大于0.02wt%时,BSA在TEMPDMAEMA网格单元内表现出从垂直取向到平面取向(H-P)的变化,此时BSA和PDMAEMA的电荷状态分别为负和正。然而,对于其他pI高于PDMAEMA的pKa的蛋白质,由于它们相同的阳离子电荷产生的静电排斥,这种取向变化并未发生。该结果表明,蛋白质与PDMAEMA之间的静电相互作用是通过TEMPDMAEMA网格单元内的H-P转变进行蛋白质检测的主要贡献因素。DNA是一种与pH无关的强阴离子聚电解质,也用TEMPDMAEMA网格单元进行了测试,并且在PDMAEMA的电荷状态低于其pKa阈值且浓度高于0.01wt%时表现出H-P转变。因此,我们证明了TEMPDMAEMA网格单元通过使用偏振光学显微镜的H-P转变有效地促进了带负电荷的生物材料(即蛋白质和DNA)的检测。这种用于非特异性生物材料检测的简单且廉价的实验装置为开发使用聚电解质的有效生物传感器奠定了基础。

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