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Ab65347

Manufactured by Abcam
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Ab65347 is a lab equipment product from Abcam. It is a device used for the measurement and analysis of specific components or characteristics in a sample. The core function of this product is to provide accurate and reliable data to support scientific research and laboratory experiments.

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Lab products found in correlation

Zen microscope software, by Zeiss (2 mentions) Tr22421, by Fujifilm (2 mentions) Hr series nefa hr 2, by Fujifilm (2 mentions) Tr13421, by Fujifilm (2 mentions) Tr15408, by Fujifilm (2 mentions) Evos xl, by Zeiss (2 mentions) Ab199082, by Abcam (1 mentions) Ab65390, by Abcam (1 mentions) Ab65336, by Abcam (1 mentions) Mak002, by Merck Group (1 mentions)

3 protocols using ab65347

1

Metabolic profiling and atherosclerosis quantification

Cited 2 times
Check if the same lab product or an alternative is used in the 5 most similar protocols
Serum metabolites (cholesterol, triglycerides, glucose, free fatty
acids) were assayed from blood obtained from mice after 6-hour fast per
manufacturer’s protocols (Thermo Scientific TR13421, TR22421, TR15408,
and Wako Diagnostics HR Series NEFA-HR(2)).
For glucose tolerance test, mice were fasted for 6 hours, injected with
10% D-glucose (1 g/kg), and tail vein blood obtained at different time points
was analyzed using a glucometer (Contour, Bayer Healthcare, Mishawaka, IN).
Serum L-amino acid were measured from mice fed standard or high protein
Western diets for 2 month or from fasted mice given an oral protein gavage for
the indicated time points using a colorimetric L-amino acid assay kit (Abcam,
ab65347) following the manufacturer’s protocol.
Quantification of atherosclerosis at the aortic root was as
follows12 (link),21 (link). PBS-perfused hearts were placed in a
cryostat mold containing tissue freezing medium. 10 μm thick sections
were taken from the samples beginning just caudal to the aortic sinus and
extending into the proximal aorta. Slides were fixed with 4% paraformaldehyde
and stained with Oil Red O. Images were taken by EVOS XL Core Cell Imaging
system and Oil Red O positive regions were quantified using ZEN microscope
software (Carl Zeiss AG).
Zhang X., Sergin I., Evans T.D., Jeong S.J., Rodriguez-Velez A., Kapoor D., Chen S., Song E., Holloway K.B., Crowley J.R., Epelman S., Weihl C.C., Diwan A., Fan D., Mittendorfer B., Stitziel N.O., Schilling J.D., Lodhi I.J, & Razani B. (2020). High-protein diets increase cardiovascular risk by activating macrophage mTOR to suppress mitophagy. Nature metabolism, 2(1), 110-125.
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2

Metabolic profiling and atherosclerosis quantification

Cited 2 times
Check if the same lab product or an alternative is used in the 5 most similar protocols
Serum metabolites (cholesterol, triglycerides, glucose, free fatty
acids) were assayed from blood obtained from mice after 6-hour fast per
manufacturer’s protocols (Thermo Scientific TR13421, TR22421, TR15408,
and Wako Diagnostics HR Series NEFA-HR(2)).
For glucose tolerance test, mice were fasted for 6 hours, injected with
10% D-glucose (1 g/kg), and tail vein blood obtained at different time points
was analyzed using a glucometer (Contour, Bayer Healthcare, Mishawaka, IN).
Serum L-amino acid were measured from mice fed standard or high protein
Western diets for 2 month or from fasted mice given an oral protein gavage for
the indicated time points using a colorimetric L-amino acid assay kit (Abcam,
ab65347) following the manufacturer’s protocol.
Quantification of atherosclerosis at the aortic root was as
follows12 (link),21 (link). PBS-perfused hearts were placed in a
cryostat mold containing tissue freezing medium. 10 μm thick sections
were taken from the samples beginning just caudal to the aortic sinus and
extending into the proximal aorta. Slides were fixed with 4% paraformaldehyde
and stained with Oil Red O. Images were taken by EVOS XL Core Cell Imaging
system and Oil Red O positive regions were quantified using ZEN microscope
software (Carl Zeiss AG).
Zhang X., Sergin I., Evans T.D., Jeong S.J., Rodriguez-Velez A., Kapoor D., Chen S., Song E., Holloway K.B., Crowley J.R., Epelman S., Weihl C.C., Diwan A., Fan D., Mittendorfer B., Stitziel N.O., Schilling J.D., Lodhi I.J, & Razani B. (2020). High-protein diets increase cardiovascular risk by activating macrophage mTOR to suppress mitophagy. Nature metabolism, 2(1), 110-125.
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3

Plasma Metabolite Profiling Using ELISA

Check if the same lab product or an alternative is used in the 5 most similar protocols
Plasma total amino acids were measured using fluorometric-based ELISA kits as described (MAK002, Sigma-Aldrich, Ab65347, Abcam). Plasma FGF21 was measured using a fluorescent based ELISA kit (ab229382, Abcam). Plasma triglyceride, cholesterol and leptin were measured using ELISA kits (ab65336, ab65390, ab199082, Abcam). Individual amino acids were measured using Gas Chromatography/Mass Spectrometry (WellChild laboratory, Evelina Children’s Hospital, St Thomas’s Hospital, London).
Hope D.C., Hinds C.E., Lopes T., Vincent M.L., Shrewsbury J.V., Yu A.T., Davies I., Scott R., Jones B., Murphy K.G., Minnion J.S., Sardini A., Carling D., Lutz T.A., Bloom S.R., Tan T.M, & Owen B.M. (2022). Hypoaminoacidemia underpins glucagon-mediated energy expenditure and weight loss. Cell Reports Medicine, 3(11), 100810.
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