Quantitative PCR Protocol for Gene Expression

RNA isolation from cells and tissues and subsequent reverse transcription were performed as described in [32 (link)]. Quantitative real-time PCR was performed by applying LightCycler technology (Roche Diagnostics, Mannheim, Germany) while using specific sets of primers, as listed in Table 1. For normalization, the amplification of cDNA derived from β-actin was carried out.

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Sommer J., Ehnis H., Seitz T., Schneider J., Wild A.B., Moceri S., Buechler C., Bozec A., Weber G.F., Merkel S., Beckervordersandforth R., Steinkasserer A., Schüle R., Trebicka J., Hartmann A., Bosserhoff A., von Hörsten S., Dietrich P, & Hellerbrand C. (2023). Four-and-a-Half LIM-Domain Protein 2 (FHL2) Induces Neuropeptide Y (NPY) in Macrophages in Visceral Adipose Tissue and Promotes Diet-Induced Obesity. International Journal of Molecular Sciences, 24(19), 14943.

Publication 2023

LightCycler technology

Actin Cdna Cells isolation Diagnostics Primers Quantitative real time pcr Reverse transcription Tissues

Corresponding Organization :

Other organizations : Friedrich-Alexander-Universität Erlangen-Nürnberg, Universitätsklinikum Erlangen, University Hospital Regensburg, University Medical Center Freiburg, University of Freiburg, University of Münster

Top 5 similar protocols

Variable analysis

independent variables

RNA isolation from cells and tissues
Reverse transcription

dependent variables

Quantitative real-time PCR

control variables

Amplification of cDNA derived from β-actin for normalization

controls

Positive control: Not explicitly mentioned
Negative control: Not explicitly mentioned

Annotations

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