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Peptide Sequencing- The Edman Degradation

With the identities and relative amounts of amino acids known, a peptide can then be sequenced to find out in what order the amino acids are linked. Much peptide sequencing is now done by mass spectrometry, using either electrospray ionization (ESI) or matrix-assisted laser desorption ionization (MALDI) linked to a time-of-flight (TOF) mass analyzer, as described in Section 12.4. Also in common use is a chemical method of peptide sequencing called the Edman degradation.

The general idea of peptide sequencing by Edman degradation is to cleave one amino acid at a time from an end of the peptide chain. That terminal amino acid is then separated and identified, and the cleavage reactions are repeated on the chain-shortened peptide until the entire peptide sequence is known. Automated protein sequencers are available that allow as many as 50 repetitive sequencing cycles to be carried out before a buildup of unwanted by-products interferes with the results. So efficient are these instruments that sequence information can be obtained from as little as 1 to 5 picomoles of sample—less than 0.1 μg.

As shown in Figure 26.5, Edman degradation involves treatment of a peptide with phenyl isothiocyanate (PITC), C6H5–N═C═, followed by reaction with trifluoroacetic acid. The first step attaches the PITC to the –NH2 group of the N-terminal amino acid, and the second step splits the N-terminal residue from the peptide chain, yielding an anilinothiazolinone (ATZ) derivative plus the chain-shortened peptide. Further acid-catalyzed rearrangement of the ATZ derivative with aqueous acid converts it into a phenylthiohydantoin (PTH), which is identified by comparison of its elution time with the known elution times of PTH derivatives of the 20 common amino acids. The chain-shortened peptide is then automatically resubmitted for another round of Edman degradation.

Figure 26.5 MECHANISM Mechanism of the Edman degradation for N-terminal analysis of peptides.
Peptide Sequencing- The Edman Degradation | Chemistry Optional Notes for UPSCPeptide Sequencing- The Edman Degradation | Chemistry Optional Notes for UPSC

Complete sequencing of large proteins by Edman degradation is impractical because of the buildup of unwanted by-products. To get around this problem, a large peptide chain is first cleaved by partial hydrolysis into a number of smaller fragments, the sequence of each fragment is determined, and the individual fragments are fitted together by matching their overlapping ends. In this way, protein chains with more than 400 amino acids have been sequenced.

Partial hydrolysis of a peptide can be carried out either chemically with aqueous acid or enzymatically. Acid hydrolysis is unselective and gives a more-or-less random mixture of small fragments, but enzymatic hydrolysis is quite specific. The enzyme trypsin, for instance, catalyzes hydrolysis of peptides only at the carboxyl side of the basic amino acids arginine and lysine; chymotrypsin cleaves only at the carboxyl side of the aryl-substituted amino acids phenylalanine, tyrosine, and tryptophan.
Peptide Sequencing- The Edman Degradation | Chemistry Optional Notes for UPSC

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FAQs on Peptide Sequencing- The Edman Degradation - Chemistry Optional Notes for UPSC

1. What is peptide sequencing?
Ans. Peptide sequencing is the process of determining the order of amino acids in a peptide or protein molecule. It is a crucial step in understanding the structure and function of these molecules.
2. What is the Edman degradation method?
Ans. The Edman degradation is a widely used method for sequencing peptides. It involves selectively removing one amino acid at a time from the N-terminus (starting end) of the peptide and analyzing it to determine its identity. This process is repeated iteratively to sequence the entire peptide.
3. How does the Edman degradation work?
Ans. In the Edman degradation, the peptide is first reacted with phenylisothiocyanate (PITC) to form a phenylthiocarbamoyl (PTC) derivative. This derivative is then selectively cleaved from the N-terminus using anhydrous trifluoroacetic acid (TFA). The released PTC-amino acid can then be analyzed using techniques such as chromatography or mass spectrometry.
4. What are the limitations of the Edman degradation method?
Ans. The Edman degradation method has certain limitations. It is time-consuming as each amino acid needs to be removed and analyzed individually. It is also limited to peptides of moderate length (around 50-70 amino acids) and may not be suitable for complex protein molecules. Additionally, certain amino acids, such as proline, can cause difficulties in the degradation process.
5. Are there alternative methods for peptide sequencing?
Ans. Yes, there are alternative methods for peptide sequencing, such as mass spectrometry-based approaches. These methods involve fragmenting the peptide into smaller pieces and analyzing the resulting fragments to determine their sequence. Mass spectrometry-based methods offer advantages such as higher throughput and the ability to analyze larger proteins, but they may require additional computational analysis for accurate sequencing.
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