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Application of Hanging Drop Technique for Kidney Tissue Culture.


ABSTRACT: The hanging drop technique is a well-established method used in culture of animal tissues. However, this method has not been used in adult kidney tissue culture yet. This study was to explore the feasibility of using this technique for culturing adult kidney cortex to study the time course of RNA viability in the tubules and vasculature, as well as the tissue structural integrity.In each Petri dish with the plate covered with sterile buffer, a section of mouse renal cortex was cultured within a drop of DMEM culture medium on the inner surface of the lip facing downward. The tissue were then harvested at each specific time points for Real-time PCR analysis and histological studies.The results showed that the mRNA level of most Na+ related transporters and cotransporters were stably maintained within 6 hours in culture, and that the mRNA level of most receptors found in the vasculature and glomeruli were stably maintained for up to 9 days in culture. Paraffin sections of the cultured renal cortex indicated that the tubules began to lose tubular integrity after 6 hours, but the glomeruli and vasculatures were still recognizable up to 9 days in culture.We concluded that adult kidney tissue culture by hanging drop method can be used to study gene expressions in vasculature and glomeruli.

SUBMITTER: Wang S 

PROVIDER: S-EPMC6050513 | biostudies-literature | 2017

REPOSITORIES: biostudies-literature

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Application of Hanging Drop Technique for Kidney Tissue Culture.

Wang Shaohui S   Wang Ximing X   Boone Jasmine J   Wie Jin J   Yip Kay-Pong KP   Zhang Jie J   Wang Lei L   Liu Ruisheng R  

Kidney & blood pressure research 20170504 2


<h4>Background/aims</h4>The hanging drop technique is a well-established method used in culture of animal tissues. However, this method has not been used in adult kidney tissue culture yet. This study was to explore the feasibility of using this technique for culturing adult kidney cortex to study the time course of RNA viability in the tubules and vasculature, as well as the tissue structural integrity.<h4>Methods</h4>In each Petri dish with the plate covered with sterile buffer, a section of m  ...[more]

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