Minimized cell usage for stem cell-derived and primary cells on an automated patch clamp system

Nadine Becker; Sonja Stoelzle; Sven Göpel; David Guinot; Patrick Mumm; Claudia Haarmann; Daniela Malan; Heribert Bohlen; Eugen Kossolov; Ralf Kettenhofen; Michael George; Niels Fertig; Andrea Brüggemann

doi:10.1016/j.vascn.2013.03.009

Minimized cell usage for stem cell-derived and primary cells on an automated patch clamp system

J Pharmacol Toxicol Methods. 2013 Jul-Aug;68(1):82-7. doi: 10.1016/j.vascn.2013.03.009. Epub 2013 Apr 6.

Authors

Nadine Becker¹, Sonja Stoelzle, Sven Göpel, David Guinot, Patrick Mumm, Claudia Haarmann, Daniela Malan, Heribert Bohlen, Eugen Kossolov, Ralf Kettenhofen, Michael George, Niels Fertig, Andrea Brüggemann

Affiliation

¹ Nanion Technologies GmbH, Gabrielenstraße 9, 80636 Munich, Germany. nadine@nanion.de

PMID: 23567076
DOI: 10.1016/j.vascn.2013.03.009

Abstract

Introduction: Chip-based automated patch clamp systems are widely used in drug development and safety pharmacology, allowing for high quality, high throughput screening at standardized experimental conditions. The merits of automation generally come at the cost of large amounts of cells needed, since cells are not targeted individually, but randomly positioned onto the chip aperture from cells in suspension. While cell usage is of little concern when using standard cell lines such as CHO or HEK cells, it becomes a crucial constraint with cells of limited availability, such as primary or otherwise rare and expensive cells, like induced pluripotent stem (IPS) cell-derived cardiomyocytes or neurons.

Methods: We established application protocols for CHO cells, IPS cell-derived neurons (iCell® Neurons, Cellular Dynamics International), cardiomyocytes (Cor.4U®, Axiogenesis) and pancreatic islet cells, minimizing cell usage for automated patch clamp recordings on Nanion's Patchliner. Use of 5 μl cell suspension per well for densities between 55,000 cells/ml and 400,000 cells/ml depending on cell type resulted in good cell capture.

Results: We present a new cell application procedure optimized for the Patchliner achieving>80% success rates for using as little as 300 to 2000 cells per well depending on cell type. We demonstrate that this protocol works for standard cell lines, as well as for stem cell-derived neurons and cardiomyocytes, and for primary pancreatic islet cells. We present recordings for these cell types, demonstrating that high data quality is not compromised by altered cell application.

Discussion: Our new cell application procedure achieves high success rates with unprecedentedly low cell numbers. Compared to other standard automated patch clamp systems we reduced the average amount of cells needed by more than 150 times. Reduced cell usage crucially improves cost efficiency for expensive cells and opens up automated patch clamp for primary cells of limited availability.

Keywords: Automated patch clamp; Patchliner; pancreatic islet cells; primary cells; stem cell-derived cardiomyocytes; stem cell-derived neurons.

Publication types

Comparative Study

MeSH terms

Animals
Automation
CHO Cells / cytology
Cricetinae
Cricetulus
Humans
Induced Pluripotent Stem Cells / cytology*
Islets of Langerhans / cytology
Mice
Myocytes, Cardiac / cytology*
Neurons / cytology*
Patch-Clamp Techniques / economics
Patch-Clamp Techniques / methods*