Nanodrop 0nec microvolume uv vis spectrophotometer

Manufactured by Thermo Fisher Scientific

The NanoDrop™ One Microvolume UV–Vis Spectrophotometer is a compact and versatile instrument designed for the measurement of small sample volumes. It utilizes a patented sample retention system that allows for the analysis of sample sizes as low as 0.5 μL. The instrument provides accurate and reliable absorbance measurements across a wide wavelength range, enabling the quantification and quality assessment of various biomolecules, including nucleic acids and proteins.

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2 protocols using nanodrop 0nec microvolume uv vis spectrophotometer

Osteogenic Potential of Fibromodulin in mSSC

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FACS-isolated mSSC were harvested from DO Den and DO Inn specimens at POD 10 and cultured in 96 well plates over a course of 10 days in osteogenic medium with media changes every 48 h in duplicates. Cells were treated with and without a single dose of hFibromodulin (FMOD) protein (0.1 mg/ml, R&D 9840-FM-050) at 12 h to evaluate the ability of FMOD to augment osteogenic potential. The monolayer of cells was fixed with 100% ethanol for 15 min and stained with alizarin red solution for 1 h at room temperature. The cells were washed several times with ultrapure water and imaged for osteogenic potential immediately. Following imaging, the cells were treated with a methanol/acetic acid mixture for 15 min and absorbance was detected at 450 nm using NanoDrop™ 0ne^c Microvolume UV–Vis Spectrophotometer (ThermoFisher)^{12 (link)}.

Tevlin R., Griffin M., Chen K., Januszyk M., Guardino N., Spielman A., Walters S., Gold G.E., Chan C.K., Gurtner G.C., Wan D.C, & Longaker M.T. (2023). Denervation during mandibular distraction osteogenesis results in impaired bone formation. Scientific Reports, 13, 2097.

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Osteogenic Potential of Mandible mSSCs

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FACS-isolated mSSC harvested from uninjured and POD10 mandibles were cultured in 96-well plates over a course of two weeks at low-oxygen conditions, then incubated with osteogenic medium for an additional two weeks with media changes every 48 hours. The cells were then washed with PBS and ultra-pure water and fixed with 100% ethanol. Cells were then stained with alizarin red solution at room temperature. Cells were washed with ultra-pure water and imaged immediately. After imaging, the cells were incubated with methanol/acetic acid mixture and alizarin red protein concentration was detected at 450 nm using NanoDrop™ 0ne^c Microvolume UV-Vis Spectrophotometer (ThermoFisher). Values from uninjured, innervated P0D10 and denervated P0D10 mandible defects were compared using ANOVA.

Jones R.E., Salhotra A., Robertson K.S., Ransom R.C., Foster D.S., Shah H.N., Quarto N., Wan D.C, & Longaker M.T. (2019). Skeletal Stem Cell-Schwann Cell Circuitry in Mandibular Repair. Cell reports, 28(11), 2757-2766.e5.

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