Abstract

BackgroundSolid-state micropores have been widely employed for 6 decades to recognize and size flowing unlabeled cells. However, the resistive-pulse technique presents limitations when the cells to be differentiated have overlapping dimension ranges such as B and T lymphocytes. An alternative approach would be to specifically capture cells by solid-state micropores. Here, the inner wall of 15-µm pores made in 10 µm-thick silicon membranes was covered with antibodies specific to cell surface proteins of B or T lymphocytes. The selective trapping of individual unlabeled cells in a bio-functionalized micropore makes them recognizable just using optical microscopy.Methodology/Principal FindingsWe locally deposited oligodeoxynucleotide (ODN) and ODN-conjugated antibody probes on the inner wall of the micropores by forming thin films of polypyrrole-ODN copolymers using contactless electro-functionalization. The trapping capabilities of the bio-functionalized micropores were validated using optical microscopy and the resistive-pulse technique by selectively capturing polystyrene microbeads coated with complementary ODN. B or T lymphocytes from a mouse splenocyte suspension were specifically immobilized on micropore walls functionalized with complementary ODN-conjugated antibodies targeting cell surface proteins.Conclusions/SignificanceThe results showed that locally bio-functionalized micropores can isolate target cells from a suspension during their translocation throughout the pore, including among cells of similar dimensions in complex mixtures.

Highlights

  • Purification and analysis of a distinct cell type depend on the previous isolation of a particular cell subpopulation from a heterogeneous cell mixture

  • Separation of the cells according to surface markers is of particular interest to provide highly purified populations, especially via immunolabeling of a cluster of differentiation (CD) with a fluorophore or a magnetic bead for Fluorescent Activated Cell Sorting (FACS) [3] and magnetic separation [4], respectively

  • Specific isolation of the cells of interest using antibodies immobilized on a solid surface has been exploited in Cell-Affinity Chromatography (CAC) devices [5,6,7,8,9] and protein arrays [10,11,12,13,14]

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Summary

Introduction

Purification and analysis of a distinct cell type depend on the previous isolation of a particular cell subpopulation from a heterogeneous cell mixture. Conclusions/Significance: The results showed that locally bio-functionalized micropores can isolate target cells from a suspension during their translocation throughout the pore, including among cells of similar dimensions in complex mixtures. Cell surface protein-specific antibodies conjugated with complementary ODNs were immobilized on the pore walls via hybridization.

Results
Conclusion

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