Protein sequencing


Digestion into peptide fragments


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Protein sequencing - Wikipedia

Digestion into peptide fragments
Peptides longer than about 50–70 amino
acids long cannot be sequenced reliably
by the Edman degradation. Because of
this, long protein chains need to be
broken up into small fragments that can


then be sequenced individually. Digestion
is done either by endopeptidases such as
trypsin or pepsin or by chemical reagents
such as cyanogen bromide. Different
enzymes give different cleavage
patterns, and the overlap between
fragments can be used to construct an
overall sequence.
Reaction
The peptide to be sequenced is adsorbed
onto a solid surface. One common
substrate is glass fibre coated with
polybrene, a cationic polymer. The
Edman reagent, phenylisothiocyanate
(PITC), is added to the adsorbed peptide,


together with a mildly basic buffer
solution of 12% trimethylamine. This
reacts with the amine group of the N-
terminal amino acid.
The terminal amino acid can then be
selectively detached by the addition of
anhydrous acid. The derivative then
isomerises to give a substituted
phenylthiohydantoin, which can be
washed off and identified by
chromatography, and the cycle can be
repeated. The efficiency of each step is
about 98%, which allows about 50 amino
acids to be reliably determined.


Protein sequencer
protein sequenator 
[3]
is a machine that
performs Edman degradation in an
automated manner. A sample of the
protein or peptide is immobilized in the
reaction vessel of the protein sequenator
and the Edman degradation is
performed. Each cycle releases and
derivatises one amino acid from the
protein or peptide's N-terminus and the
A Beckman-Coulter Porton LF3000G protein sequencing machine


released amino-acid derivative is then
identified by HPLC. The sequencing
process is done repetitively for the whole
polypeptide until the entire measurable
sequence is established or for a pre-
determined number of cycles.
Protein identification is the process of
assigning a name to a protein of interest
(POI), based on its amino-acid sequence.
Typically, only part of the protein’s
sequence needs to be determined
experimentally in order to identify the
protein with reference to databases of
protein sequences deduced from the
Identification by mass
spectrometry


DNA sequences of their genes. Further
protein characterization may include
confirmation of the actual N- and C-
termini of the POI, determination of
sequence variants and identification of
any post-translational modifications
present.

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