1. Academic Validation
  2. Development of a CD63 Aptamer for Efficient Cancer Immunochemistry and Immunoaffinity-Based Exosome Isolation

Development of a CD63 Aptamer for Efficient Cancer Immunochemistry and Immunoaffinity-Based Exosome Isolation

  • Molecules. 2020 Nov 27;25(23):5585. doi: 10.3390/molecules25235585.
Zhenguo Song 1 Jun Mao 2 Roberto A Barrero 3 Peng Wang 4 Fengqiu Zhang 5 Tao Wang 4
Affiliations

Affiliations

  • 1 Department of Pharmacy, Affiliated Cancer Hospital of Zhengzhou University, Zhengzhou 450008, China.
  • 2 College of Basic Medical Sciences, Dalian Medical University, Dalian 116044, China.
  • 3 eResearch Office, Division of Research and Innovation, Queensland University of Technology, Brisbane City QLD 4001, Australia.
  • 4 College of Nursing and Health, Zhengzhou University, Zhengzhou 450001, China.
  • 5 Henan Key Laboratory of Ion-beam Bioengineering, Zhengzhou University, Zhengzhou 450000, China.
Abstract

CD63, a member of transmembrane-4-superfamily of tetraspanin proteins and a highly N-glycosylated type III lysosomal membrane protein, is known to regulate malignancy of various types of cancers such as melanoma and breast Cancer and serves as a potential marker for Cancer detection. Recently, its important role as a classic exosome marker was also emphasized. In this work, via using a magnetic bead-based competitive SELEX (systematic evolution of ligands by exponential enrichment) procedure and introducing a 0.5M NaCl as elution buffer, we identified two DNA Aptamers (CD63-1 and CD63-2) with high affinity and specificity to CD63 protein (Kd = 38.71nM and 78.43, respectively). Furthermore, CD63-1 was found to be efficient in binding CD63 positive cells, including breast Cancer MDA-MB-231 cells and CD63-overexpressed HEK293T cells, with a medium binding affinity (Kd~ 100 nM) as assessed by flow cytometry. When immunostaining assay was performed using clinical breast Cancer biopsy, the CD63-1 aptamer demonstrated a comparable diagnostic efficacy for CD63 positive breast Cancer with commercial Antibodies. After developing a magnetic bead-based exosome immunoaffinity separation system using CD63-1 aptamer, it was found that this bead-based system could effectively isolate exosomes from both MDA-MB-231 and HT29 Cell Culture medium. Importantly, the introduction of the NaCl elution in this work enabled the isolation of native exosomes via a simple 0.5M NaCl incubation step. Based on these results, we firmly believe that the developed Aptamers could be useful towards efficient isolation of native state exosomes from clinical samples and various theranostic applications for CD63-positive cancers.

Keywords

CD63; SELEX; aptamer; breast cancer; cancer; exosome.

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