A facile approach to the isolation of proteins in Ferula asafoetida and their enzyme stabilizing, anti-microbial and anti-oxidant activity

The objective of the present study was to identify the proteome pattern, isolate and study the functions of selective proteins from Ferula asafoetida root exudate using chromatographic techniques. The root exudate proteins were fractionated using ion-exchange and gel filtration chromatography. A ran...

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Bibliographic Details
Published in:International journal of biological macromolecules 2017-09, Vol.102, p.1211-1219
Main Authors: Chandran, Sanjana, Sakthivel, Meenakumari, Thirumavalavan, Munusamy, Thota, Jagadeshwar Reddy, Mariappanadar, Vairamani, Raman, Pachaiappan
Format: Article
Language:English
Subjects:
Anti-bacterial
Anti-Infective Agents - chemistry
Anti-Infective Agents - isolation & purification
Anti-Infective Agents - pharmacology
Anti-oxidant
Antioxidants - chemistry
Antioxidants - isolation & purification
Antioxidants - pharmacology
Asafoetida
Chemical Fractionation - methods
Chymotrypsin - metabolism
Enzyme stability
Enzyme Stability - drug effects
Ferula - chemistry
Molecular Weight
Plant Proteins - chemistry
Plant Proteins - isolation & purification
Plant Proteins - pharmacology
Plant Roots - chemistry
Proteins
Trypsin - metabolism
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Summary:The objective of the present study was to identify the proteome pattern, isolate and study the functions of selective proteins from Ferula asafoetida root exudate using chromatographic techniques. The root exudate proteins were fractionated using ion-exchange and gel filtration chromatography. A range of bioactive protein fractions were then separated in sufficient quantity which is the focus of this study. Based on studies, here we report three main proteins with molecular weights 14kDa, 27kDa, and 39kDa. The biological and pharmacological activities of both purified and unpurified proteins obtained were extensively studied to understand their significance. The study revelaed that 27kDa protein interestingly stabilized trypsin activity in 24h of time and retained about 64% of the enzyme activity. Analyses confirmed 40°C and pH 8.0 are the optimum temperature and pH respectively. The 39kDa protein remarkably increased the activity of chymotrypsin and the 14kDa protein showed anti-bacterial activity against Pseudomonas aeruginosa. Invariably all of the three purified proteins showed enhanced anti-oxidant activity. In conclusion, results here obtained suggested that the primary metabolites (proteins) in asafoetida are mainly responsible for its versatile biological and pharmacological activities.
ISSN:0141-8130
1879-0003
DOI:10.1016/j.ijbiomac.2017.05.010