A bead-based immunogold-silver staining assay on capillary-driven microfluidics

被引:11
|
作者
Pham, Ngoc M. [1 ]
Rusch, Sebastian [2 ,3 ,4 ]
Temiz, Yuksel [5 ]
Lovchik, Robert D. [5 ]
Beck, Hans-Peter [2 ,3 ]
Karlen, Walter [1 ]
Delamarche, Emmanuel [5 ]
机构
[1] ETH, Mobile Hlth Syst Lab, Inst Robot & Intelligent Syst, Dept Hlth Sci & Technol,BAA, Lengghalde 5, CH-8092 Zurich, Switzerland
[2] Swiss Trop & Publ Hlth Inst, Socinstr 57, CH-4051 Basel, Switzerland
[3] Univ Basel, Petersgraben 1, CH-4001 Basel, Switzerland
[4] Kantonsspital Aarau AG, Inst Lab Med, Med Genet, Tellstr 25, CH-5001 Aarau, Switzerland
[5] IBM Res Zurich, Saumerstr 4, CH-8803 Ruschlikon, Switzerland
基金
瑞士国家科学基金会;
关键词
Microfluidics; Silver staining; Immunoassays; Microbeads; IMMUNOSORBENT-ASSAY; GOLD NANOPARTICLES; DETECTION SYSTEMS; RUBELLA-VIRUS; IMMUNOASSAY; BIOMARKERS; ANTIBODIES; CHIP;
D O I
10.1007/s10544-018-0284-6
中图分类号
R318 [生物医学工程];
学科分类号
0831 ;
摘要
Point-of-care (POC) diagnostics are critically needed for the detection of infectious diseases, particularly in remote settings where accurate and appropriate diagnosis can save lives. However, it is difficult to implement immunoassays, and specifically immunoassays relying on signal amplification using silver staining, into POC diagnostic devices. Effective immobilization of antibodies in such devices is another challenge. Here, we present strategies for immobilizing capture antibodies (cAbs) in capillary-driven microfluidic chips and implementing a gold-catalyzed silver staining reaction. We illustrate these strategies using a species/anti-species immunoassay and the capillary assembly of fluorescent microbeads functionalized with cAbs in "bead lanes", which are engraved in microfluidic chips. The microfluidic chips are fabricated in silicon (Si) and sealed with a dry film resist. Rabbit IgG antibodies in samples are captured on the beads and bound by detection antibodies (dAbs) conjugated to gold nanoparticles. The gold nanoparticles catalyze the formation of a metallic film of silver, which attenuates fluorescence from the beads in an analyte-concentration dependent manner. The performance of these immunoassays was found comparable to that of assays performed in 96 well microtiter plates using "classical" enzyme-linked immunosorbent assay (ELISA). The proof-of-concept method developed here can detect 24.6 ng mL(-1) of rabbit IgG antibodies in PBS within 20 min, in comparison to 17.1 ng mL(-1) of the same antibodies using a similar to 140-min-long ELISA protocol. Furthermore, the concept presented here is flexible and necessitate volumes of samples and reagents in the range of just a few microliters.
引用
收藏
页数:9
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