Dissociation of Aβ aggregates and detection of Aβ on IME sensor

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Fig. 2 Dissociation of Aβ aggregates and detection of Aβ on IME sensor. Dissociation of Aβ aggregates and detection of Aβ on IME sensor. (A) Scheme of Aβ monomerization by EPPS treatment after spiking plasma samples with aggregated Aβ. (B to D) Changes of Aβ levels in plasma via EPPS treatment (before and after) when Aβ aggregates were spiked into human plasma. Concentrations of Aβ are 400 pg/ml (B), 200 pg/ml (C), and 100 pg/ml (D). Statistical comparisons were made with two-tailed t test: P = 0.0003 (B) and P = 0.0146 (D). Black squares, untreated samples; white squares, EPPS-treated samples. (E) IME chip and the enlarged image of one IME pair (scanning electron microscopic image). (F) Sequential process for surface modification of the IME sensor. The IME sensor was sequentially functionalized with APMES, PVP-CHO, glutaraldehyde, Aβ antibody (6E10), and BSA. (G) Image of IME sensor and PDMS microfluidic chip. Each sample was injected into two microfluidic channels on the IME unit chip. (H) IME unit chip with PDMS microfluidic chip photograph. Two channels were filled with colored solutions. (I) Impedance change (|ΔZ/Z0|, %) of the IME by interaction between Aβ and its antibody. (J) Logarithmical linear sensitivity to Aβ levels (n = 5). Error bars indicate SDs. (K and L) Analysis of mouse plasma Aβ levels [black dot, WT (n = 9); red dot, TG (n = 9)]. (K) WT mouse plasma without and with EPPS treatment. (L) TG mouse plasma without and with EPPS treatment. The dot data represent multiple (n = 5) independent experiments. Two-tailed t tests were performed in the statistical analyses (*P < 0.05 and ***P < 0.001; nonsignificant analysis is not indicated). YoungSoo Kim et al. Sci Adv 2019;5:eaav1388 Copyright © 2019 The Authors, some rights reserved; exclusive licensee American Association for the Advancement of Science. No claim to original U.S. Government Works. Distributed under a Creative Commons Attribution NonCommercial License 4.0 (CC BY-NC).