محلول برادفورد 5X حجم 100 سی سی DNAbiotech
محلول برادفورد 5X حجم 100 سی سی DNAbiotech
Bradford Reagent, 5X
Cat #: DB9701-100ml
Volume: 100ml
Sensitivity: (aprox.) 20 ugr - 1.5 mgr/ml
Package: Dark brown glass bottle
For Molecularr Biology research
Storage: 4o C
محصولات مشابه
-
فنول اشباع حجم 100 سی سی DNAbiotech
تماس بگیرید -
محلول برادفورد 5X حجم 50 سی سی DNAbiotech
235000 تومان -
فنول اشباع حجم 50 سی سی DNAbiotech
تماس بگیرید -
ستون خالی کروماتوگرافی
185000 تومان -
فنول اشباع حجم 25 سی سی DNAbiotech
تماس بگیرید -
RNA Stabilization solution محلول پایدار کننده RNA حجم 100ml
560000 تومان -
مستر میکس real time PCR با راکس High ROX biofact sybr master mix
تماس بگیرید -
RNA Stabilization solution 25 ml محلول پایدار کننده RNA حجم 25ml
195000 تومان -
مستر میکس real time PCR کم راکس Biofact
ناموجود -
RNA Stabilization solution 50ml محلول پایدار کننده RNA حجم 50ml
295000 تومان -
مستر میکس real time PCR بدون راکس Biofact
ناموجود -
آنتی هیومن کونژوگه با HRP حجم 100 میکرولیترDNAbiotech
1850000 تومان -
استریپ qPCR حجم 0.1 ml برند Gunster Biotech بسته 12 تایی
395000 تومان -
آنتی هیومن کونژوگه با HRP حجم 500 میکرولیترDNAbiotech
4900000 تومان -
استریپ qPCR حجم 0.1 ml برند Gunster Biotech جعبه
3500000 تومان -
رزین نیکل NTA حجم 1 سی سی
880000 تومان -
کیت استخراج RNA توتال پارس (خون، بافت و سلول) 50 واکنشی
2550000 تومان -
رزین نیکل NTA حجم 5 سی سی
3650000 تومان -
کیت سوبسترای ECL پارس حجم 100 سی سی
1350000 تومان -
محلول متوقف کننده الایزا ELISA stop solution
185000 تومان -
کیت سوبسترای ECL پارس حجم 50 سی سی
695000 تومان -
IPTG پنج گرمی DNAbiotech
2950000 تومان -
کیت سوبسترای DAB حجم 100ml برند DNAbiotech
تماس بگیرید -
IPTG یک گرمی DNAbiotech
680000 تومان -
کیت BCA حجم 100 سی سی (BCA 100 ml) برای 1330 واکنش سرمایشی
1790000 تومان
Bradford Reagent
Notes:
- The change in the color of Coomassie G-250 from red to blue upon binding protein is measured spectroscopically. In the absence of protein, when the dye is red, Bradford reagent has an absorbance maximum (Amax) of 470 nm.
- A standard curve, also known as a calibration curve, is a type of graph used as a quantitative research technique. Multiple samples with known properties are measured and graphed, which then allows the same properties to be determined for unknown samples by interpolation on the graph
- BSA is used because of its stability to increase signal in assays, its lack of effect in many biochemical reactions, and its low cost, since large quantities of it can be readily purified from bovine blood, a byproduct of the cattle industry.
Many protein-containing solutions have the highest absorption at 280 nm in the spectrophotometer, the UV range. This requires spectrophotometers capable of measuring in the UV range, which many cannot. Additionally, the absorption maxima at 280 nm requires that proteins contain aromatic amino acids such as tyrosine (Y), phenylalanine (F) and/or tryptophan (W). Not all proteins contain these amino acids, a fact which will skew the concentration measurements. If nucleic acids are present in the sample, they would also absorb light at 280 nm, skewing the results further. By using the Bradford protein assay, one can avoid all of these complications by simply mixing the protein samples with the Coomassie Brilliant Blue G-250 dye (Bradford reagent) and measuring their absorbances at 595 nm, which is in the Vis range.
The procedure for Bradford protein assay is very easy and simple to follow. It is done in one step where the Bradford reagent is added to a test tube along with the sample. After mixing well, the mixture almost immediately changes to a blue color. When the dye binds to the proteins through a process that takes about 2 minutes, a change in the absorption maximum of the dye from 465 nm to 595 nm in acidic solutions occurs. This dye creates strong noncovalent bonds with the proteins, via electrostatic interactions with the amino and carboxyl groups, as well as Van Der Waals interactions. Only the molecules that bind to the proteins in solution exhibit this change in absorption, which eliminates the concern that unbound molecules of the dye might contribute to the experimentally obtained absorption reading. This process is more beneficial since it is less pricey than other methods, easy to use, and has high sensitivity of the dye for protein
نظرات کاربران