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  • Combining whole-cell patch clamp and dye loading in acute brain slices with bulk RNA sequencing in embryonic to aged mice.

Combining whole-cell patch clamp and dye loading in acute brain slices with bulk RNA sequencing in embryonic to aged mice.

STAR protocols (2021-04-27)
Yasmine Kamen, Ragnhildur Thóra Káradóttir
ABSTRACT

Single-cell electrophysiological recordings combined with dye loading and immunohistochemistry provide unparalleled single-cell resolution of cell physiology, morphology, location, and protein expression. When correlated with bulk RNA sequencing, these data can define cell identity and function. Here, we describe a protocol to prepare acute brain slices from embryonic and postnatal mice for whole-cell patch clamp, dye loading and post-hoc immunohistochemistry, and cell isolation for bulk RNA sequencing. While we focus on oligodendrocyte precursor cells, this protocol is applicable to other brain cells. For complete details on the use and execution of this protocol, please refer to Spitzer et al. (2019).

MATERIALI
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Potassio cloruro, ACS reagent, 99.0-100.5%
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Acido cloridrico, ACS reagent, 37%
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Fosfato di sodio, ACS reagent, ≥98%
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HEPES, ≥99.5% (titration)
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Triton X-100, for molecular biology
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Glicina, suitable for electrophoresis, ≥99%
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DAPI, for nucleic acid staining
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Desossiribonucleasi I, Type IV, lyophilized powder, ≥2,000 Kunitz units/mg protein
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2-mercaptoetanolo, ≥99.0%
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Siero di capra
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Guanosina 5′-trifosfato, ≥95% (HPLC), powder
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Adenosina 5′-trifosfato, ≥95%, bacterial
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D-(+)-Glucosio, ≥99.5% (GC), BioXtra
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