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Enzychrom sialic acid assay kit

Manufactured by BioAssay Systems
Sourced in United States

The EnzyChrom Sialic Acid Assay Kit is a colorimetric assay that quantifies sialic acid in biological samples. It uses a two-step enzymatic reaction to produce a colored product that can be measured spectrophotometrically.

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5 protocols using enzychrom sialic acid assay kit

1

Quantifying Sialic Acid Content

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Bound sialic acid content was obtained using EnzyChrom Sialic Acid Assay Kit (BioAssay Systems). TA muscle lysates were either treated with a hydrolysis reagent (1 h at 80 °C) for cleavage of bound sialic acid content or used untreated to measure free sialic acid. The samples were placed in black clear - bottom 96-well plates, probed with dye reagent and the enzyme provided by the kit. The amount of sialic acid of the samples was measured in excitation wavelength of 535 nm and emission wavelength of 595 nm, and compared to a 0 to 500 pmol sialic acid standard curve.
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2

Serum Sialic Acid Quantification

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Level of serum total sialic acid was measured by using EnzyChrom™ Sialic Acid Assay Kit (cat# ESLA-100) (Bioassay system, Inc., USA) according to the protocol of manufacturer.
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3

Quantification of Sialic Acid in Fc-Glycoproteins

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The quantification of sialic acid content in the purified Fc-fusion glycoproteins was performed through an EnzyChrom Sialic Acid Assay Kit (BioAssay Systems, Hayward, CA, USA) and a Sialic Acid Quantitation Kit (Agilent Technologies, Santa Clara, CA, USA).
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4

Sialic Acid Quantification in Mouse Urine

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The total sialic acid content in mouse urine was measured using the Enzychrom Sialic Acid Assay Kit, according to the manufacturer’s instructions (BioAssay Systems, Hayward, CA, USA).
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5

Purification and Analysis of Recombinant EPO

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The recombinant EPO secreted into the cell culture medium was puri ed by reversed-phase chromatography (Yoon et al. 2005) (link). EPO was separated from culture supernatant by loading the samples onto a reversed-phase column (RESOURCE RPC 3 mL, GE Healthcare). The EPO was separated from the samples by utilizing gradient elution: eluent A was composed of 10 mM Tris (pH 7), and eluent B was composed of 10 mM Tris and 80% ethanol (pH 7). The peak related to EPO was observed at a concentration of 65% ethanol, and SDS-PAGE and Western blot assessed the purity of obtained EPO. Then, the buffer of puri ed EPO protein was exchanged with deionized water through the dialysis process at 4 o C.
Determination of glucose, ammonia, lactate, and EPO sialic acid contents
The glucose content of samples was determined by an enzymatic assay kit (Abcam, USA), as per kit instructions. Ammonia concentration was measured based on an ammonia detection kit (Sigma-Aldrich, USA) regarding the instruction manual. According to kit instructions, lactate determination was conducted based on a lactate assay kit (R-Biopharm, Germany). The sialic acid content of puri ed EPO was determined by utilizing the EnzyChrom sialic acid assay kit (BioAssay Systems, CA), following the manufacturer's protocol.
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