Intravital imaging of the kidney

Hato, Takashi; Winfree, Seth; Dagher, Pierre C.

Intravital imaging of the kidney

Files

If you need an accessible version of this item, please email your request to digschol@iu.edu so that they may create one and provide it to you.

Date

2017-09-01

Authors

Hato, Takashi

Winfree, Seth

Dagher, Pierre C.

Language

American English

Department

Medicine, School of Medicine

Found At

Elsevier

Abstract

Two-photon intravital microscopy is a powerful tool that allows the examination of dynamic cellular processes in the live animal with unprecedented resolution. Indeed, it offers the ability to address unique biological questions that may not be solved by other means. While two-photon intravital microscopy has been successfully applied to study many organs, the kidney presents its own unique challenges that need to be overcome in order to optimize and validate imaging data. For kidney imaging, the complexity of renal architecture and salient autofluorescence merit special considerations as these elements directly impact image acquisition and data interpretation. Here, using illustrative cases, we provide practical guides and discuss issues that may arise during two-photon live imaging of the rodent kidney.

Keywords

intravital microscopy, kidney, renal architecture

Cite As

Hato, T., Winfree, S., & Dagher, P. C. (2017). Intravital imaging of the kidney. Methods (San Diego, Calif.), 128, 33–39. https://doi.org/10.1016/j.ymeth.2017.03.024

ISSN

1046-2023

Journal

Methods (San Diego, Calif.)

Rights

Publisher Policy

Source

PMC

Type

Article

Permanent Link

https://hdl.handle.net/1805/15378

DOI

https://doi.org/10.1016/j.ymeth.2017.03.024

Version

Author's manuscript

Collections

Open Access Policy Articles
Department of Medicine Works

Full item page