A novel imaging method for quantitative Golgi localization reveals differential intra-Golgi trafficking of secretory cargoes

Author:

Tie Hieng Chiong1,Mahajan Divyanshu1,Chen Bing1,Cheng Li23,VanDongen Antonius M. J.4,Lu Lei1

Affiliation:

1. School of Biological Sciences, Nanyang Technological University, Singapore 637551

2. Bioinformatics Institute, Singapore 138671

3. School of Computing, National University of Singapore, Singapore 117417

4. Program in Neuroscience and Behavioral Disorders, Duke-NUS Graduate Medical School, Singapore 169857

Abstract

Cellular functions of the Golgi are determined by the unique distribution of its resident proteins. Currently, electron microscopy is required for the localization of a Golgi protein at the sub-Golgi level. We developed a quantitative sub-Golgi localization method based on centers of fluorescence masses of nocodazole-induced Golgi ministacks under conventional optical microscopy. Our method is rapid, convenient, and quantitative, and it yields a practical localization resolution of ∼30 nm. The method was validated by the previous electron microscopy data. We quantitatively studied the intra-Golgi trafficking of synchronized secretory membrane cargoes and directly demonstrated the cisternal progression of cargoes from the cis- to the trans-Golgi. Our data suggest that the constitutive efflux of secretory cargoes could be restricted at the Golgi stack, and the entry of the trans-Golgi network in secretory pathway could be signal dependent.

Publisher

American Society for Cell Biology (ASCB)

Subject

Cell Biology,Molecular Biology

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