商品編號:P0144600304803 原始貨號:K-SUFRG
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蔗糖/果糖/葡萄糖檢測套組 Sucrose/D-Fructose/D-Glucose Assay Kit

Megazyme台灣區正式授權總代理
產品編號: No.  700004342
目錄編號: No.  K-SUFRG
  • 用於測量樣品中蔗糖、果糖、葡萄糖的含量
  • 此套組樣品來源適用於酒類、果汁、軟性飲料、牛奶、乳製品、肉類製品、果醬、蜂蜜、烘培食品、嬰兒食品、糖類製品、糖果、巧克力、點心、冰淇淋、蔬果、菸草、化妝品、調味品和其他材料(例如:生物培養材料)...等
  • 檢測原理:
    1️⃣蔗糖含量➡️樣品中的蔗糖經酵素(β-Fructosidase)作用,會被分解成單糖(葡萄糖、果糖)。此時葡萄糖再次經過酵素(Hexokinase、Glucose-6-phosphate dehydrogenase)作用後結構發生轉變,最後其產物為gluconate-6-phosphate和NADPH。分光光度計(spectrophotometer)在340 nm的波長下,可檢測NADPH產生之吸光值(NADP+ 不會產生吸光值),後續再與標準溶液之吸光值對照,即可得到測試結果。比對蔗糖分解前後葡萄糖之濃度差異,即可計算出蔗糖含量
    2️⃣D-葡萄糖含量➡️樣品中的葡萄糖經過酵素(Hexokinase、Glucose-6-phosphate dehydrogenase)作用後結構發生轉變,最後其產物為gluconate-6-phosphate和NADPH。分光光度計(spectrophotometer)在340 nm的波長下,可檢測NADPH產生之吸光值(NADP+ 不會產生吸光值),後續再與標準溶液之吸光值對照,即可得到測試結果。
    3️⃣D-果糖含量(僅限 D-葡萄糖/D-果糖樣品)➡️樣品中的果糖透過酵素會轉變為葡萄糖-6-磷酸(glucose-6-phosphate),葡萄糖-6-磷酸經過酵素(Glucose-6-phosphate dehydrogenase)作用後結構發生轉變,最後其產物為gluconate-6-phosphate和NADPH。分光光度計(spectrophotometer)在340 nm的波長下,可檢測NADPH產生之吸光值(NADP+ 不會產生吸光值),後續再與標準溶液之吸光值對照,即可得到測試結果。樣品的吸光度差值減去空白對照組的吸光度差值,即可得到樣品的果糖含量。
  • 此套組之測量結果,需搭配分光光度計(spectrophotometer)使用
  • 偵測極限: 1.38 mg/L
  • 線性範圍: 4 to 80 µg of D-glucose, D-fructose or sucrose per assay
  • 便捷、易用、易學、易上手
  • 節省設備建置、實驗室空間、耗材、委外送驗等開銷
  • 提供線上可下載之計算工具,原始數據輕鬆處理
  • 總測試時間:約23分鐘
  • 應用:食品研發、學術研究、原物料和成品檢驗
  • 冷藏(2–8°C)可短期存放,如需長時間保存,請參考瓶身的保存方式(酵素保存方式皆不相同)
     
  • 供應規格:300   檢測反應 
    ➡️(蔗糖、果糖、葡萄糖各100個檢測反應)
  • 供應規格:此套組內僅提供酵素溶液,其他藥品及耗材需另購
  • 國際認證:
    基於此原理之檢測方法,已被NF, EN, NEN, DIN, GOST, IFU, AIJN, MEBAK and IOCCC 所接受
     
  • 此商品交期約30-45天,可接受在下單。
  •     7天鑑賞期後即可折抵
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  • 原價 : $ 9,999,999

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商品特色

  • 操作流程(PROCEDURE)




     
  • 樣品準備(SAMPLE PREPARATION)
    1.  Sample dilution.
    The amount of sugar (D-glucose plus D-fructose plus sucrose) present in the cuvette (i.e. in the 0.1 mL of sample being analysed) should range between 4 and 80 μg.  The sample solution must therefore be diluted sufficiently to yield a sugar concentration between 0.04 and 0.8 g/L.

    2.  Sample clarification.

    a.  Solutions:
    Carrez I solution.  Dissolve 3.60 g of potassium hexacyanoferrate (II) {K4[Fe(CN)6].3H2O} (Sigma cat. no. P9387) in 100 mL of distilled water.  Store at room temperature.
    Carrez II solution.  Dissolve 7.20 g of zinc sulphate (ZnSO4.7H2O)  (Sigma cat. no. Z4750) in 100 mL of distilled water.  Store at room temperature.
    Sodium hydroxide (NaOH, 100 mM).  Dissolve 4 g of NaOH in 1 L of distilled water.  Store at room temperature.

    b.  Procedure:
    Pipette the liquid sample into a 100 mL volumetric flask which contains approx. 60 mL of distilled water, or weigh sufficient quantity of the sample into a 100 mL volumetric flask and add 60 mL of distilled water.  Carefully add 5 mL of Carrez I solution, 5 mL of Carrez II solution and 10 mL of NaOH solution (100 mM).  Mix after each addition.  Fill the volumetric flask to the mark, mix and filter.

    3.  General considerations.
    (a)  Liquid samples: clear, slightly coloured and approximately neutral, liquid samples can be used directly in the assay.
    (b)  Acidic samples: if > 0.1 mL of an acidic sample is to be used undiluted (such as wine or fruit juice), the pH of the solution should be increased to approx. 7.6 using 2 M NaOH, and the solution incubated at room temperature for 30 min.
    (c)  Carbon dioxide: samples containing a significant amount of carbon dioxide, such as beer, should be degassed by increasing the pH to approx. 7.6 with 2 M NaOH and gentle stirring, or by stirring with a glass rod.
    (d)  Coloured samples: an additional sample blank, i.e. sample with no HK/G6P-DH, may be necessary in the case of coloured samples.
    (e)  Strongly coloured samples: if used undiluted, strongly coloured samples should be treated by the addition of 0.2 g of polyvinylpolypyrrolidone (PVPP)/10 mL of sample.  Shake the tube vigorously for 5 min and then filter through Whatman No. 1 filter paper.
    (f)  Solid samples: homogenise or crush solid samples in distilled water and filter if necessary.
    (g)  Samples containing fat: extract such samples with hot water at a temperature above the melting point of the fat, e.g. in a 100 mL volumetric flask.  Adjust to 20°C and fill the volumetric flask to the mark with water.  Store on ice or in a refrigerator for 15-30 min and then filter.  Discard the first few mL of filtrate and use the clear supernatant (which may be slightly opalescent) for assay.  Alternatively, clarify with Carrez reagents.
    (h)  Samples containing protein: deproteinise samples containing protein with Carrez reagents.

商品規格

  • 商品規格(300個檢測反應)
    ➡️(蔗糖、果糖、葡萄糖各100個檢測反應)

  • Bottle 1:  
    Buffer 1 (25 mL, pH 7.6) plus sodium azide   (0.02% w/v) as a preservative. 
    Stable for > 2 years at 4°C.

    Bottle 2: 
    NADP+ plus ATP.   
    Stable for > 5 years below -10°C.
     
    Bottle 3: 
    Hexokinase plus glucose-6-phosphate dehydrogenase suspension, (4.1 mL).     
    Stable for > 2 years at 4°C.

    Bottle 4: 
    Phosphoglucose isomerase suspension (2.25 mL).     
    Stable for > 2 years at 4°C.

    Bottle 5: 
    D-Glucose plus D-fructose standard solution   (5 mL, 0.2 mg/mL of each sugar).   
    Stable for > 2 years at 4°C.

    Bottle 6: 
    β-Fructosidase (pH 4.6), lyophilised powder.   
    Stable for > 2 years below -10°C.

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