A method and kit for stable enzymatic detection of sialic acid
A kit and sialic acid technology, which is applied in the field of enzymatic detection of sialic acid, can solve the problems of short stabilization time, inability to meet clinical detection needs, short stabilization period, etc.
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Embodiment 1
[0084] Embodiment 1 adopts the SA detection kit of single reagent
[0085] The reagent of the kit adopts a single reagent, and the components and concentrations of the reagents are as follows:
[0086] Neuraminidase 50KU / L
[0087] Neuraminic acid aldolase 50KU / L
[0088] Oxidized coenzyme NAD0.1mmol / L
[0089] Mannosamine dehydrogenase 50KU / L
[0090] MES buffer 100mmol / L
[0091] Polyethylene glycol 0.05%
[0092] Sodium Azide 0.05%
[0093] The pH of the reagent is 7.0, where the stated percentages are weight to volume.
[0094] The method of using a single reagent is as follows:
[0095] Table 1: How to use a single reagent
[0096]
sample
standard blank
standard
[0097] serum
60ul
standard
60ul
60ul
Reagent I
1800ul
1800ul
1800ul
[0098] Mix well and react at 37°C for 10 minutes, adjust to zero with pure water, and measure the absorbance change of each tube. ...
Embodiment 2
[0102] Embodiment 2 adopts the SA detection kit of double reagent
[0103] The kit’s reagents use dual reagents, and the components and concentrations of reagent 1 are as follows:
[0104] Neuraminidase 80KU / L
[0105] Oxidized coenzyme NAD4mmol / L
[0106] HEPES buffer 100mmol / L
[0107] Polyethylene glycol 0.1%
[0108] Sodium Benzoate 0.1%
[0109] Reagent 1 has a pH of 6.5, where the percentages are weight to volume.
[0110] The composition and concentration of reagent 2 are as follows:
[0111] Neuraminic acid aldolase 10KU / L
[0112] Mannosamine dehydrogenase 60KU / L
[0113] HEPES buffer 400mmol / L
[0114] Glycerol 5%
[0115] Sodium Azide 0.1%
[0116] Reagent 2 has a pH of 7.2, where the percentages are weight to volume.
[0117] The dual reagents are used as follows:
[0118] Table 2: How to use the dual reagents
[0119]
[0120]
[0121] Mix well and react at 37°C for 10 minutes, adjust to zero with pure water, and measure the absorbance change of...
Embodiment 3
[0125]Embodiment 3 adopts the SA detection kit of double reagent
[0126] The kit’s reagents use dual reagents, and the components and concentrations of reagent 1 are as follows:
[0127] Neuraminidase 100KU / L
[0128] Oxidized coenzyme NAD4mmol / L
[0129] HEPES buffer 100mmol / L
[0130] Polyethylene glycol 0.1%
[0131] Sodium Benzoate 0.1%
[0132] Reagent 1 has a pH of 6.5, where the percentages are weight to volume.
[0133] The composition and concentration of reagent 2 are as follows:
[0134] Neuraminic acid aldolase 10KU / L
[0135] Mannosamine dehydrogenase 100KU / L
[0136] HEPES buffer 400mmol / L
[0137] Glycerol 5%
[0138] Sodium Azide 0.1%
[0139] Reagent 2 has a pH of 7.2, where the percentages are weight to volume.
[0140] Its usage method is as the kit in Example 2.
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