General-purpose acetylcholinesterase activity colorimetric quantitative detection kit instructions

Universal acetylcholinesterase activity colorimetric quantitative detection kit product specification (Chinese)

The main purpose

The universal acetylcholinesterase activity colorimetric quantitative detection reagent is a product designed to release thiol choline through an acetylcholinesterase reaction system, and a yellow 5-mercapto-2-nitrobenzoic acid product is produced using an Ellman reagent. The change in the peak absorbance, the authoritative and classical technical method of determining the enzyme activity in a sample by colorimetry. The technology has been carefully developed and successfully tested. It is suitable for the detection of acetylcholinesterase activity in samples of various animals and human cells, tissues, blood, body fluids and the like. The product is strictly sterile, ready to use, simple in operation and stable in performance.

technical background

Acetylcholinesterase (AchE; EC 3.1.1.7), also known as erythrocyte cholinesterase, is widely found in eukaryotes, including certain plants, especially in brain tissue, neuromuscular junctions ( Neuromuscular junction), central nervous system cholinergic synapses and erythrocyte membranes are highly expressed, catalyzing the hydrolysis of the main neurotransmitter acetylcholine, producing acetic acid and choline, and terminating synaptic transmission. Its function is to regulate the action of acetylcholine. Neurotoxic gases, such as organophosphate (Sarin), inhibit acetylcholinesterase activity, cause neuromuscular spasm, and eventually asphyxiation. The serum acetylcholinesterase concentration is significantly reduced in association with organophosphorus pesticide poisoning, so blood testing is an important indicator of environmental pollution. Based on the synthetic substrate iodide thiothiocholine iodide, under the action of acetylcholinesterase, hydrolyzed to produce acetic acid and thiocholine, and Ellman reagent 5,5-dithio-bis(2-nitrate After the reaction of [5,5'-dithiobis-(2-nitrobenzoic acid); DTNB], a yellow 5-thio-2-nitrobenzoic acid (TNB) is produced. The activity of acetylcholinesterase was quantitatively analyzed by the change in its absorption peak (wavelength at 412 nm). The acetylcholinesterase reaction system is:

Acetylcholinesterase

Acetylthiocholine iodide → acetate + thiocholine

DTNB + thiocholine → TNB + choline-SS-TNB

product content

Buffer (Reagent A) 20 ml

Reaction solution (Reagent B) 1 ml

Substrate solution (Reagent C) 2 ml

Negative solution (Reagent D) 1 ml

Product manual 1 copy

storage method

Store in a -20 ° C refrigerator; Reagent B and Reagent C to avoid light; effective June

User-supplied

Cuvette or 96-well plate: a container for colorimetry

Spectrophotometer or microplate reader: for colorimetric analysis

Experimental procedure

  • Preparation for measurement

  • Prepare the sample to be tested and place it in the ice tank.
  • Turn on and set up the spectrophotometer (temperature is 37 ° C): wavelength 412nm, interval 5 minutes, reading 3 times (15 minutes total), and set zero
  • Reagents removed from -20 ℃ refrigerator, an ice melting trough; reaction solution (Reagent B) and substrate solution (Reagent C) protected from light
  • The buffer (Reagent A ) is equilibrated at room temperature; the substrate solution (Reagent C ) is incubated at 50 ° C.

  • Sample background control

  • Transfer 190 μl of buffer (Reagent A ) to the new cuvette
  • Add 25 μl of negative solution (Reagent D )
  • Add 25 μl of substrate solution (Reagent C )
  • Pour up and down several times and mix
  • Incubate for 3 minutes at 37 ° C
  • Add 10 μl of the sample to be tested (20 μg of protein) (Note: the sample should be clear )
  • Pour up and down several times, mix (limited to 3 seconds)
  • Immediately put into the spectrophotometer test, this is the sample background control (15 minutes reading - 0 minutes reading)

  • Sample determination

  • Transfer 190 μl of buffer (Reagent A ) to the new cuvette
  • Add 25 μl of reaction solution (Reagent B )
  • Add 25 μl of substrate solution (Reagent C )
  • Pour up and down several times and mix
  • Incubate for 3 minutes at 37 ° C
  • Add 10 μl of the sample to be tested (20 μg of protein) (Note: the sample should be clear )
  • Pour up and down several times, mix (limited to 3 seconds)
  • Immediately put into the spectrophotometer test, this is the sample reading (15 minutes reading - 0 minutes reading)

Fourth, calculate sample activity

[(Sample reading - background reading) X 0.25 (system capacity; ml) X sample dilution factor] ÷ [0.01 (sample capacity; ml) X 13.6 (mmol absorbance) X 15 (reaction time; minutes)] = unit / ÷ ÷ (sample protein concentration) mg / ml = unit / mg

Unit = micromolar thiocholine / minute

Five, microplate reader determination

  • Mark the corresponding on the 96-well plate: sample background control and sample to be tested
  • Transfer 190 μl of buffer (Reagent A ) to a 96-well plate.
  • Add 25 μl of negative solution (Reagent D ) to the sample control well
  • Add 25 μl of reaction solution (Reagent B ) to the sample well to be tested
  • Add 25 μl of substrate solution (Reagent C ) to all wells
  • Gently shake the 96-well plate
  • Incubate for 3 minutes at 37 ° C
  • Add 10 μl of the sample to be tested (20 μg protein) to all wells (note: the sample should be clear )
  • Gently shake the 96-well plate
  • Immediately put into the microplate reader test: 0 minute reading and 15 minute reading
  • Activity calculation:

[(Sample reading - background reading) X sample dilution factor X 0.25 (system capacity; ml)] ÷ [0.01 (sample capacity; ml) X 13.6 (mmol absorbance) X 0.6 (light path distance; cm) X 15 ( Reaction time; minutes)] = unit / ml ÷ (sample protein concentration) mg / ml = unit / mg

Unit = micromolar thiocholine / minute

Precautions

  • This product is 50 operations
  • Wear gloves when handling
  • Background determination for each sample
  • It is recommended to use cuvette determination
  • Samples must be clarified, it is vital
  • Colorimetric determination within 3 seconds after loading
  • The measured value changes from low to high; the measurement lasts for 15 minutes.
  • After the colorimetric determination, the cuvette must be thoroughly cleaned.
  • The sample is measured for 15 minutes and the reading is higher than 0 minutes.
  • It is recommended that the sample protein concentration to be tested be 20 μg/10 μl (the company provides Bradford Protein Concentration Quantitation Kit -30030.1)
  • If the concentration of the sample to be tested is too high or too low, the sample concentration can be adjusted.
  • Acetylcholinesterase unit activity is defined as the amount of enzyme required to produce 1 micromole of thiocholine per minute at 37 ° C, pH 7.5 as an active unit
  • The company provides a series of acetylcholinesterase detection reagent products

Quality Standard

  • This product has been certified to be stable.
  • This product has been identified and sensitive

Single Packed Yellow Waxy Corn Cob

For the most common waxy and sweet corn on the market, waxy corn has a higher nutrient content than regular corn, containing 70-75% starch (and almost all straight-chain starch), more than 10% protein, 4-5% fat and 2% multivitamins, with more grains, VA, VB1 and VB2 in protein than rice, with the highest fat and VB2 content. Yellow maize also contains carotenoids, such as rice and wheat. The molecular weight of waxy maize starch is more than 10 times smaller than that of ordinary maize, and the starch makes glutinous rice sticky and soft, softer than ordinary hard maize. It is more than 20% more digestible to eat than regular maize and it is suitable for people with less than perfect teeth. At the same time, it is not suitable for diabetics because of the very high content of straight-chain starch (a polysaccharide).

Waxy maize is also known as sticky maize. The grain has coarse, waxy endosperm, similar to shiny, glassy (clear) grains such as hard and dent maize. Its chemical and physical characteristics are controlled by a recessive gene, which is located on chromosome 9. 100% of the starch in the endosperm is straight-chain starch.

Single Packed Waxy Corn Cob

975t05975t04

If you have any further questions about our products, please do not hesitate to contact us.

Waxy Corn Cob,Yellow Glutinous Corn,Yellow Waxy Corn Cob,Single Packed Yellow Waxy Corn Cob

Jilin Province Argricultural Sister-in-law Food Co., Ltd. , https://www.nongsaocorns.com