Steroid Probes Conjugated with Protein-Protected Gold Nanocluster: Specific and Rapid Fluorescence Imaging of Steroid Receptors in Target Cells

Chi-Yan Tsai; Chun-Wei Li; Jie-Ren Li; Bo-Han Jang; Shu-Hui Chen

doi:10.1007/s10895-016-1811-6

Steroid Probes Conjugated with Protein-Protected Gold Nanocluster: Specific and Rapid Fluorescence Imaging of Steroid Receptors in Target Cells

J Fluoresc. 2016 Jul;26(4):1239-48. doi: 10.1007/s10895-016-1811-6. Epub 2016 May 10.

Authors

Chi-Yan Tsai¹, Chun-Wei Li², Jie-Ren Li¹, Bo-Han Jang¹, Shu-Hui Chen³

Affiliations

¹ Department of Chemistry, National Cheng Kung University, Tainan, Taiwan.
² Department of Medical Imaging and Radiological Sciences, College of Health Science, Kaohsiung Medical University, Kaohsiung, Taiwan. cwl0331@gmail.com.
³ Department of Chemistry, National Cheng Kung University, Tainan, Taiwan. shchen@mail.ncku.edu.tw.

PMID: 27165037
DOI: 10.1007/s10895-016-1811-6

Abstract

Steroid ligands can easily diffuse through the cell membrane and this property makes it feasible to be used for in-situ staining of the nuclear receptors. However, nonspecific binding of the internalized ligand probe with the cellular components has caused serious interferences for the detection of receptor-expressing cells. We report a novel gold nanocluster (AuNC)-conjugated estrogen probe that can eliminate nonspecific internalization and accelerate nuclear localization to achieve selective and rapid detection of estrogen receptors (ERs) in live cells. The AuNC, protected by bovine serum albumin (BSA), BSA-AuNCs, was prepared by the synthesis and confirmed to be 1.9 nm in core size and 18 nm in diameter. Ethinyl estradiol was used as the precursor of 17β-estradial (E2) to conjugate with BSA-protected AuNCs via polyethylene glycol linker (E2-PEG/BSA-AuNCs) or to conjugate with Cy3 dyes (E2-Cy3). The conjugated probe was determined to contain five E2 molecules per BSA-AuNC by mass spectrometry and exhibit an emission maximum of around 640 nm, which was not altered by E2 conjugation indicating that the structural integrity of BSA-AuNCs was conserved. E2-PEG/BSA-AuNCs probes were quickly internalized by MCF-7 (ER+) cells and localized to the nuclei in 2 h. Such internalization was sensitive to competition by free E2 and was rarely detected in the controls using either non-conjugated BSA-AuNCs in MCF-7 (ER+) cells or E2-PEG/BSA-AuNCs in MDA-MB-231 (ER-) cells. In contrast to the high specificity of E2-PEG/BSA-AuNCs probe, the uptake of E2-Cy3 probe could not differentiate between MCF-7(ER+) and MDA-MB-231(ER-) cells during the early phases of the treatment. Moreover, nuclear targeting by E2-Cy3 was three times slower than that by the E2-PEG/BSA-AuNC probe. Such accelerated nuclei targeting was consistent with the enhanced cell viability by conjugating E2 with BSA-AuNC. In conclusion, the E2-PEG/BSA-AuNC probes are promising candidates that can be used for the detection of ER+ tumor tissues and the same strategy can be applied to fabricate other steroid probes.

Keywords: Estrogen; Estrogen receptor; Gold nanoclusters; Steroid probe.

MeSH terms

Alkynes / chemistry
Animals
Biological Transport
Carbocyanines / chemistry
Cattle
Cell Survival
Click Chemistry
Estradiol / chemistry*
Estradiol / metabolism
Ethinyl Estradiol / chemistry
Gold / chemistry*
Humans
MCF-7 Cells
Metal Nanoparticles / chemistry*
Optical Imaging / methods*
Receptors, Estrogen / metabolism*
Serum Albumin, Bovine / chemistry*

Substances

Alkynes
Carbocyanines
Receptors, Estrogen
cyanine dye 3
Serum Albumin, Bovine
Ethinyl Estradiol
Estradiol
Gold