Coordination Chemistry of a Controlled Burst of Zn2+ in Bulk Aqueous and Nanosized Water Droplets with a Zincon Chelator.

Abstract

The light-induced photolysis of [Zn(NTAdeCage)]- generates a temporally controlled burst of Zn2+, which is rapidly chelated in situ by the free ligand Zincon2-. The [Zn(Zincon)]2- coordination progress is monitored using absorption spectroscopy in bulk aqueous buffer and reverse micelle environments. The [Zn(NTAdeCage)]- photocage and free ligand Zincon2- have different reverse micelle locations that affect the [Zn(Zincon)]2- formation at the nanoscale compared to the bulk aqueous buffer. The formation of [Zn(Zincon)]2- in a bulk aqueous buffer is more efficient despite the released Zn2+ and Zincon2- being physically closer within reverse micelles. The observed reduction of complex formation is attributed to the interfacial partitioning of Zincon2-, distinct from the Zn2+ photocage in the water pool, requiring diffusion for the species to meet to form [Zn(Zincon)]2-. This work introduces a proof-of-concept methodology to experimentally measure fast chelation reactions in confined spaces and thus provides an approach to exploring cellular responses.