Recording electrical currents across the plasma membrane of mammalian sperm cells

Boheng Liu, Nadine Mundt, Melissa Miller, David E. Clapham, Yuriy Kirichok, Polina V. Lishko

Research output: Contribution to journalArticlepeer-review

6 Scopus citations

Abstract

Recording of the electrical activity from one of the smallest cells of a mammalian organism-a sperm cell-has been a challenging task for electrophysiologists for many decades. The method known as "spermatozoan patch clamp" was introduced in 2006. It has enabled the direct recording of ion channel activity in whole-cell and cell-attached configurations and has been instrumental in describing sperm cell physiology and the molecular identity of various calcium, potassium, sodium, chloride, and proton ion channels. However, recording from single spermatozoa requires advanced skills and training in electrophysiology. This detailed protocol summarizes the step-by-step procedure and highlights several 'tricks-of-the-trade' in order to make it available to anyone who wishes to explore the fascinating physiology of the sperm cell. Specifically, the protocol describes recording from human and murine sperm cells but can be adapted to essentially any mammalian sperm cell of any species. The protocol covers important details of the application of this technique, such as isolation of sperm cells, selection of reagents and equipment, immobilization of the highly motile cells, formation of the tight (Gigaohm) seal between a recording electrode and the plasma membrane of the sperm cells, transition into the whole-spermatozoan mode (also known as break-in), and exemplary recordings of the sperm cell calcium ion channel, CatSper, from six mammalian species. The advantages and limitations of the sperm patch clamp method, as well as the most critical steps, are discussed.

Original languageEnglish
Article numbere62049
Pages (from-to)1-32
Number of pages32
JournalJournal of Visualized Experiments
Volume2021
Issue number168
DOIs
StatePublished - 2021

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