DK <
d...@no.email.thankstospam.net> wrote:
> In article <
mailman.236.136545...@net.bio.net>, Sudheer Sangeetham <
sudhee...@gmail.com> wrote:
> >Hello all
> >
> >I would like to quantify the protein concentration. I checked the nanodrop
> >manual in that they have given that I can estimate the protein by measuring
> >directly at 280 nm by giving extinction coefficient value without doing
> >bradford or lowry methods. I would like to choose measuring the protein
> >concentration directly. Because I need to handle many samples all the time,
> >so it is difficult for me to do bradford or lowry methods all the time. So
> >How far is correct if I estimate the protein concentration directly? please
> >give me your suggestion
> To expand on Nick's answer a bit:
> 1. If your protein is quite pure, A280 + theoretical extinction coefficient
> given by Protparam will *usually* get you as close to the real concentration
> as almost anything else (quantitative amino acid analysis is still a golden
> standatd but it's almost a lost art that few can execute competently and
> reliably these days).
> 2. If your protein is not very pure - particularly if contaminated by nucleic
> acids or large amounts of small molecules that absorb UV strongly, then
> just about anything else is going to be much more accurate than A280.
To expand a little more:
If the machine can reliably meassure at 205 nm that is the absorbtion
maximum of the peptide bond. Takes care of the problem with a protein
mixture. Small molecules and the buffer used might still pose a problem.
--
Kaj