| Description | Pyruvate Kinase (PK, EC 2.7.1.40) is widely present in animals, plants, microorganisms, and cultured cells. It catalyzes the final step of glycolysis and is one of the key rate-limiting enzymes in glycolysis, as well as a crucial enzyme for ATP production. Therefore, determining PK activity is of Pyruvate Kinase (PK, EC 2.7.1.40) is widely present in animals, plants, microorganisms, and cultured cells. It catalyzes the final step of glycolysis and is one of the key rate-limiting enzymes in glycolysis, as well as a crucial enzyme for ATP production. Therefore, determining PK activity is of significant importance.Detection Principle: PK catalyzes the conversion of phosphoenolpyruvate and ADP to ATP and pyruvate. Lactate dehydrogenase (LDH) further catalyzes the reaction of NADH and pyruvate to produce lactate and NAD⁺. The change in NADH absorbance at 340 nm is measured to calculate the PK activity in the sample.Applicable Samples: Animal/plant tissues, cells, bacteria, serum (plasma)A1501205Component48T96TStorageA1501205AExtraction Buffer60 mL60 mL×22-8℃A1501205BAssay Buffer12 mL24 mL2-8℃A1501205CSubstrate Mix1EA1EA-20℃. Store in the dark.A1501205DLDH10.2 µL20.4 µL2-8℃Please check the quantity of each component before the experiment.An additional 10% of each component is provided beyond the specified volume for standard curve preparation or preliminary experiments.User-Provided Instruments and ReagentsTypeNameNotesInstrumentMicroplate ReaderCapable of measuring absorbance at 340 nm.Consumables96-well UV PlateUV-transparent plate.ReagentsPBS (pH 7.4) / Deionized WaterFor washing cells/bacteria / Reagent preparation.OthersHomogenizer (for tissue samples), incubator, ice bucket, low-temperature centrifuge, adjustable pipettes and tipsUsing a multichannel pipette for large-scale detection can improve efficiency.Experimental Procedure1. Reagent PreparationReagent NameReagent PreparationPrecautionsExtraction BufferReady-to-use; equilibrate to room temperature before use.Store at 4°C.Assay BufferReady-to-use; equilibrate to room temperature before use.Store at 4°C.Substrate Mix Working ReagentPrepare before use: For 48T: Add 10.2 mL Assay Buffer and 0.6 mL deionized water to the vial. For 96T: Add 20.4 mL Assay Buffer and 1.2 mL deionized water to the vial. Dissolve thoroughly.After preparation, aliquot and store at -20°C for up to 6 months. Avoid repeated freeze-thaw cycles. Before use, incubate at 25°C (for general species) or 37°C (for mammals) for 5 min.LDH Working ReagentPrepare before use: For 48T: Add 0.6 mL deionized water to the LDH vial. For 96T: Add 1.2 mL deionized water to the LDH vial. Mix thoroughly.Keep on ice after preparation. The diluted reagent can be stored at 4°C for 1 month.2. Sample PreparationNote: Fresh samples are recommended. If not used immediately, samples can be stored at -80°C for up to 1 month.2.1 Animal/Plant Tissues: Weigh approximately 0.1 g of tissue, add 1 mL of Extraction Buffer, and homogenize on ice. Centrifuge at 8000 g, 4°C for 10 minutes. Collect the supernatant and keep on ice for detection.2.2 Cells/Bacteria: Collect 5×10⁶ cells or bacteria into a centrifuge tube. Wash with cold PBS, centrifuge, and discard the supernatant. Add 1 mL of Extraction Buffer. Disrupt by ultrasonic homogenization on ice (power 20% or 200 W, ultrasonicate for 3 s, interval 7 s, repeat 30 times). Centrifuge at 8000 g, 4°C for 10 minutes. Collect the supernatant and keep on ice for detection.2.3 Serum (Plasma) and other liquid samples: Detect directly.3. Assay Steps3.1 Microplate Reader Preparation: Preheat for at least 30 minutes. Set the wavelength to 340 nm.3.2 Assay System Setup: In a 96-well UV plate, add sequentially: 10 µL of sample, 10 µL of LDH Working Reagent, and 180 µL of Substrate Mix Working Reagent. Mix rapidly immediately after addition.3.3 Absorbance Measurement: Immediately after mixing, measure the absorbance at 340 nm at 20 seconds (A1) and then at 2 minutes and 20 seconds (A2). Calculate ΔA = A1 - A2.4. Result Calculation4.1 Data ProcessingCalculate ΔA = A1 - A2.4.2 Sample PK Activity Calculation(1) Based on sample mass:Unit Definition: One unit of enzyme activity is defined as the consumption of 1 nmol NADH per minute per gram of tissue in the reaction system.Formula:PK (U/g) = [ΔA×Vtotal reaction÷ (ε × d) × 10⁹] ÷ (Vsample ÷ Vtotal extract×W) ÷ T = 3215 × ΔA ÷ W(2) Based on cell/bacterial count:Unit Definition: One unit of enzyme activity is defined as the consumption of 1 nmol NADH per minute per 10⁴ bacteria or cells in the reaction system.Formula:PK (U/10⁴) = [ΔA × Vtotal reaction ÷ (ε × d) × 10⁹] ÷ (Vsample ÷ Vtotal extract; × 500) ÷ T = 3215 × ΔA ÷ 500 = 6.431 × ΔA(3) Based on liquid volume:Unit Definition: One unit of enzyme activity is defined as the consumption of 1 nmol NADH per minute per mL of serum (plasma) in the reaction system.Formula:PK (U/mL) = [ΔA × Vtotal reaction; ÷ (ε × d) × 10⁹] ÷ Vsample ÷ T = 3215 × ΔA(4) Based on protein concentration:Unit Definition: One unit of enzyme activity is defined as the consumption of 1 nmol NADH per minute per mg of protein in the reaction system.Formula:PK (U/mg prot) = [ΔA × Vtotal reaction; ÷ (ε × d) × 10⁹] ÷ (Cpr × Vsample ) ÷ T = 3215 × ΔA ÷ CprParameter Description:Vtotal reaction; : Total reaction volume, 2 × 10⁻⁴ Lε: Molar extinction coefficient of NADH, 6.22 × 10³ L/mol/cmd: Light path of the 96-well plate, 0.5 cm10⁹: Conversion factor (1 mol = 1 × 10⁹ nmol)Vsample : Volume of sample added, 0.01 mLVtotal extract; : Volume of Extraction Buffer added, 1 mLT: Reaction time, 2 minCpr: Sample protein concentration, mg/mLW: Sample mass, g500: Cell or bacterial count (5 × 10⁶), converted to units of 1Precautions1. It is recommended to perform preliminary experiments using 2-3 samples expected to have significant differences before formal testing.2. This kit is compatible with spectrophotometer detection. Adjust the preparation volume of detection reagents proportionally according to the spectrophotometer's requirements.3. For tissue and cell samples, results can be normalized by measuring the protein concentration. Aladdin BCA Protein Quantification Kit (B665595) or Ready-to-Use BCA Protein Quantification Kit (R1491648) are recommended.4. Biochemical reagents are generally irritating and biologically toxic. For your safety and health, please implement appropriate biosafety precautions throughout the experiment. Wear personal protective equipment such as lab coats, masks, gloves, and hair caps. Perform experiments in a fume hood or biosafety cabinet.5. This product is for scientific research use only. Not intended for clinical diagnosis.Frequently Asked QuestionsQ: What should I do if the sample ΔA is too high or too low?A: If the sample ΔA is > 1.0, the PK activity in the sample is too high. Dilute the sample appropriately with Extraction Buffer or reduce the amount of sample used for extraction, and then re-assay. If the sample ΔA is < 0.005, extend the reaction time to 5 or 10 minutes, or appropriately increase the sample amount, and then re-assay.Q: Will testing multiple samples simultaneously affect the results?A: Appropriately extending the time by 3-5 minutes for this assay will not affect the results. When testing multiple samples, it is recommended to use a multi-channel pipette for operation... Read More | DescriptionThe 1 µm Coupling Kit makes conducting immunoprecipitation and biomolecule separation easier and more flexible. The Kit contains AnteoBind™activated 1 µm magnetic particles that give you increased antibody binding capacity and functionality, while the included blocking DescriptionThe 1 µm Coupling Kit makes conducting immunoprecipitation and biomolecule separation easier and more flexible. The Kit contains AnteoBind™activated 1 µm magnetic particles that give you increased antibody binding capacity and functionality, while the included blocking buffer decreases background noise. Reduce reagent preparation time; remove traditional surface preparation steps such as EDC and replace these steps with the 1 µm pre-activated magnetic particles provided. This Kit reduces aggregation and gives you the freedom and ability to develop multifunctional particles for diverse applications, including dual labelling.Binding Capacity and Dispersity:Binding Capacity:> 20 µg IgG/mgMonodispersity:> 90% (by light microscopy determination)Particle based immunoassays, bioseparations and immunoprecipitation... Read More | DescriptionTruQuant IQQ is a high-quality quantitation system for making simultaneous accurate biological measurements on several hundred biochemicals in small quantities of biological samples. This is achieved by (1) spiking a complex Internal Standard (WORKFLOW-A) into a biological sample to a) DescriptionTruQuant IQQ is a high-quality quantitation system for making simultaneous accurate biological measurements on several hundred biochemicals in small quantities of biological samples. This is achieved by (1) spiking a complex Internal Standard (WORKFLOW-A) into a biological sample to a) quantify all the biochemicals in the sample relative to their counterparts in the Internal Standard, b) suppression-correct each compound and c) normalize sample to sample variances; and (2) injecting the same well characterized Long-Term Reference Standard (WORKFLOW-B) to create a daily retention time (RT) library of all compounds to be found in the Internal Standard for reproducible ID, and to measure day-to-day (QA/QC) to assure reproducible instrument performance. The system is completely automated using IROA ClusterFinder™software.IROA TruQuant IQQ Workflow Kit contains the materials and tools for the analysis of 90 experimental samples. The kit is intended to be used for mass spectrometry metabolomics applications... Read More | This reagent kit uses highly sensitive silver dye, which can be applied to protein staining of denatured and non denatured gels. It has the advantages of clear target bands, low background, and flexible control of operation time. In addition, this reagent kit has added a short-term sensitization This reagent kit uses highly sensitive silver dye, which can be applied to protein staining of denatured and non denatured gels. It has the advantages of clear target bands, low background, and flexible control of operation time. In addition, this reagent kit has added a short-term sensitization step, which can significantly reduce the background and enhance the brightness of the target band. P665901Component20 TStorageP665901ASilver Stain Sensitizer (500×)2×1 mLRTP665901BSilver Stain Enhancer3 mLRTP665901CSilver Stain2×250 mLRTP665901DSilver Stain Developer4×125 mLRT Matters needing attention1. Please prepare 50 ml of fixed solution (ultrapure water: ethanol: acetic acid=6:3:1), 50 ml of eluent (10% ethanol), and 50 ml of termination solution (5% acetic acid) in advance.2. Please use deionized water and clean glass or plastic containers during operation, and wear disposable gloves for operation.The entire silver dyeing process needs to be carried out on a shaker, with a rotation speed of about 60 rpm.4. Self prepared ethanol and glacial acetic acid are required.Instructions for useThe dosage of each solution in the following operation steps takes the gel with a size of 8.5 × 5.5 cm and a thickness of 1.0 mm as an example. The gel is immersed in the solution completely, and is operated on a shaker, with a general dosage of 25 ml. For large gel, the dosage of each solution should be scaled up according to the gel volume. Please prepare 50 ml of fixed solution (ultrapure water: ethanol: glacial acetic acid=6:3:1), 50 ml of eluent (10% ethanol), and 50 ml of termination solution (5% glacial acetic acid) in advance.1. Water washing: After electrophoresis is completed, wash the gel twice with ultrapure water for 5 minutes each time.2. Fixation: Fix the gel twice with 25 ml of fixative solution for 15 minutes each time.3. Elution: Wash the adhesive twice with eluent, each time for 5 minutes.4. Water washing: Wash the glue twice with ultrapure water, each time for 5 minutes.5. Sensitization: put the gel washed in the previous step into the silver dye sensitization working solution, incubate it accurately for 1 minute at room temperature, and then wash it with ultrapure water for three times, each time for 20 seconds. Preparation of silver staining sensitization working solution: Take 50 µ l Silver Stain Sensitivity (500 x) and add it to 25 ml of ultrapure water, mix well.6. Silver staining: discard ultrapure water and incubate gel in silver staining working solution for 30 minutes. Preparation of silver staining working solution: Take 25ml Silver Stain and add 50 µ l Silver Stain Enhanced to mix well.7. Water washing: Quickly wash the glue twice with ultrapure water, with each washing accurately controlled for 20 seconds.8. Development: Immerse the washed gel in the developer immediately and incubate it at room temperature for 2-3 minutes until the protein strip is clear. Preparation of developer: Take 25ml Silver Stain Developer and add 30 µ l Silver Stain Enhanced to mix well. Attention: Within 30 seconds of development, protein bands begin to appear and continue to develop for 2-3 minutes. If the protein band appears lighter, the development time can be appropriately extended to 5 minutes or more.9. Termination: After washing the developer on the gel with the termination solution, soak the gel in a new termination solution to react for 10 minutes.Experimental imagesSilver staining results of BSA protein samples after 10% SDS-PAGE gel electrophoresisThe molecular weight of BSA protein is about 66 kD, and the loading amounts from left to right are 50 ng, 10 ng, and 5 ng, respectively... Read More | Inquire |