A Simple Separation Method of the Protein and Polystyrene Bead-Labeled Protein for Enhancing the Performance of Fluorescent Sensor

Author:

Kim Hye Jin1,Kang Dong-Hoon2,Yang Seung-Hoon3,Lee Eunji4,Ha Taewon5,Lee Byung Chul6,Kim Youngbaek5,Hwang Kyo Seon1,Shin Hyun-Joon2,Kim Jinsik4ORCID

Affiliation:

1. Department of Clinical Pharmacology, Kyung Hee University, Seoul 02447, Republic of Korea

2. Center for Bionics, Korea Institute of Science and Technology, Seoul 02792, Republic of Korea

3. Systems Biotechnology Research Center, Korea Institute of Science and Technology, Gangneung 25451, Republic of Korea

4. Department of Medical Biotechnology, Dongguk University, Seoul 04620, Republic of Korea

5. Center for Nano-Photonics Convergence Technology, Korea Institute of Industrial Technology (KITECH), Gwangju 61012, Republic of Korea

6. Center for BioMicrosystems, Korea Institute of Science and Technology (KIST), Seoul 02792, Republic of Korea

Abstract

Dielectrophoresis- (DEP-) based separation method between a protein, amyloid beta 42, and polystyrene (PS) beads in different microholes was demonstrated for enhancement of performance for bead-based fluorescent sensor. An intensity of E2 was relative to a diameter of a microhole, and the diameters of two microholes for separation between the protein and PS beads were simulated to 3 μm and 15 μm, respectively. The microholes were fabricated by microelectromechanical systems (MEMS). The separation between the protein and the PS beads was demonstrated by comparing the average intensity of fluorescence (AIF) by each molecule. Relative AIF was measured in various applying voltage and time conditions, and the conditions for allocating the PS beads into 15 μm hole were optimized at 80 mV and 15 min, respectively. In the optimized condition, the relative AIF was observed approximately 4.908 ± 0.299. Finally, in 3 μm and 15 μm hole, the AIFs were approximately 3.143 and −1.346 by 2 nm of protein and about −2.515 and 4.211 by 30 nm of the PS beads, respectively. The results showed that 2 nm of the protein and 30 nm of PS beads were separated by DEP force in each microhole effectively, and that our method is applicable as a new method to verify an efficiency of the labeling for bead-based fluorescent sensor E2.

Funder

Dongguk University

Publisher

Hindawi Limited

Subject

Computer Science Applications,Instrumentation,General Chemical Engineering,Analytical Chemistry

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