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Mitobiogenesis in cell elisa colorimetric kit

Manufactured by Abcam

The MitoBiogenesis In-Cell ELISA Colorimetric kit is a laboratory tool used to quantify the levels of mitochondrial proteins in cell samples. It provides a colorimetric readout to measure the relative abundance of specific mitochondrial proteins within cells.

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2 protocols using mitobiogenesis in cell elisa colorimetric kit

1

Mitochondrial Protein Regulation by Idebenone

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Cells at the three stages of neural differentiation were seeded separately on a 96-well plate covered with Matrigel solution (1:30). Idebenone was added to cells for 5 days. After this time the levels of two mitochondrial proteins was measured with MitoBiogenesis In-Cell ELISA Colorimetric kit (Abcam), according to the manufacturer’s instructions, on cells fixed with 4% PFA. SDHA, mt-COX-1 proteins level was obtained on a Fluostar plate reader OMEGA (BMG Labtech). After washing with PBS, cells were incubated for 30 min in 1X Permeabilization Buffer. Prior to the addition of primary antibodies (anti-SDHA and anti-COX-1), the cells were incubated in 2X Blocking Buffer for 2 h followed by a mix of secondary antibodies conjugated with enzymes: (1) alkaline phosphatase and (2) horseradish peroxidase for 60 min. After this time substrate for alkaline phosphatase was added and absorbance was measured at OD 405 nm wavelength, then the substrate for horseradish peroxidase was added, and absorbance was measured at OD 600 nm wavelength. Changes in SDHA and COX-1 levels were normalized to total cell number measured according to manufacturer’s protocol using Janus Green (Abcam) staining method. SDHA and COX-1proteins levels were shown independently as the absorbance ratio (%) of cell samples treated by idebenone to the untreated control.
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2

Measuring Mitochondrial Biogenesis in Adipocytes

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3T3-L1 cells or human preadipocytes were plated in 24 well plates at 50,000 cells per well in 0.5 ml maintenance medium at initiation of the experiment. Mitochondrial biogenesis was measured in differentiated cells using the MitoBiogenesis In-Cell Elisa Colorimetric Kit, following the manufacturer’s protocol (Abcam). The expression of two mitochondrial proteins (COX1 and SDH) were measured simultaneously and normalized to the total protein content via JANUS staining. Absorbance (OD 600nm for COX1, OD 405nm for SDH, and OD 595nm for JANUS) was measured using a BioTek Synergy2 plate reader. The absorbance ratios of COX/SDH in experimental wells were divided by those in naïve (undifferentiated) cells, and the data are reported as “Relative Mitochondrial Protein Expression.”
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