Structural determination of improved methanol-tolerant mutant from Geobacillus zalihae T1 lipase by x-ray crystallography

Structural determination of improved methanol-tolerant mutant from Geobacillus zalihae T1 lipase by x-ray crystallography

Lipases are versatile enzymes that have been altered through various modification methods to improve their enzymatic properties to meet biotechnology industry requirement. Since decades ago, lipases from many sources have been study widely as potential biocatalyst to assist synthesis of biodiese...

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Main Author: Medam @ Hamdan, Siti Hajar
Format: Thesis
Language:English
English
Published: 2022
Subjects:
Lipase
Enzymes
X-ray crystallography
Online Access:http://psasir.upm.edu.my/id/eprint/113000/1/113000.pdf
http://psasir.upm.edu.my/id/eprint/113000/
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Institution: Universiti Putra Malaysia
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spelling my.upm.eprints.1130002024-10-24T01:06:15Z http://psasir.upm.edu.my/id/eprint/113000/ Structural determination of improved methanol-tolerant mutant from Geobacillus zalihae T1 lipase by x-ray crystallography Medam @ Hamdan, Siti Hajar Lipases are versatile enzymes that have been altered through various modification methods to improve their enzymatic properties to meet biotechnology industry requirement. Since decades ago, lipases from many sources have been study widely as potential biocatalyst to assist synthesis of biodiesel. Some of them have been altered via protein engineering approach to enhance their enzymatic performance and stability. The thermostable T1 lipase from Geobacillus zalihae can also be a great biocatalyst candidate in biodiesel production. However, inactivation of T1 lipase when the enzyme is surrounded by high concentration of methanol solvent is limiting its uses in industrial applications. Since introduction of non-bonded interactions hardly improved their stability of T1 lipase in methanol, the introduction of disulphide bond could be the best proposition to retain protein conformation and the enzyme stability in the presence of methanol. Hence, current study aims to engineer a methanoltolerant lipase by site-directed mutagenesis and divulge the interaction that stabilizes the mutant by X-ray crystallography. The preliminary study on enzyme stability was conducted by using online software ERIS, FoldX and MAESTRO. The stability of the mutant 2DC lipase was tested virtually and molecular dynamic simulation was performed in water and methanol solvent. Experimentally, the purified protein of mutant 2DC lipase was used to screen protein crystal for diffraction to elucidate and validate the mutant’s structure. It showed that the substitution of amino acid S2 and A384 with cysteine could enhance the stability of the enzyme by promoting the formation of disulphide bond to tighten the both terminal ends of the protein structure. The substitution of amino acid cysteine showed the changes on the active site distance (S113, D317, and H358), however, it was not affected the lipase activity and folding of protein structure. The 2DC mutant was successfully constructed and cloned into pET32-b and transformed into Origami B (DE3) expression host. The expression and purification using Ni2+-Sepharose affinity chromatography and gel filtration chromatography S-200 of the protein yielding 4.0 mg/ml mutant 2DC lipase suitable for protein crystallization. The mutant 2DC lipase was crystallized after 24-hour incubation at 20°C and diffracted by X-ray crystallography for deeper evaluation in term of stability and rigidity. The crystal was diffracted at 2.04 Å using in-house X-ray beam and the crystal belongs to monoclinic space group C2, with unit cell parameter of a = 118.17, b = 81.5, c = 100.05. Details information on structural elucidation of the mutant 2DC lipase has disclosed the changes within the mutant structure which associated with the alteration of enzyme activity and stability posed by the mutant. The increased in rigidity of the structure as well as changes of interaction within the catalytic region of the mutant 2DC lipase were suggested to be the factor influenced its enzymatic activity, stability and tolerance towards methanol. Hence, this newly improved mutant 2DC lipase could be the next potential biocatalyst in biodiesel production industry. 2022-10 Thesis NonPeerReviewed text en http://psasir.upm.edu.my/id/eprint/113000/1/113000.pdf Medam @ Hamdan, Siti Hajar (2022) Structural determination of improved methanol-tolerant mutant from Geobacillus zalihae T1 lipase by x-ray crystallography. Masters thesis, Universiti Putra Malaysia. Lipase Enzymes X-ray crystallography English
institution Universiti Putra Malaysia
building UPM Library
collection Institutional Repository
continent Asia
country Malaysia
content_provider Universiti Putra Malaysia
content_source UPM Institutional Repository
url_provider http://psasir.upm.edu.my/
language English
English
topic Lipase
Enzymes
X-ray crystallography
spellingShingle Lipase
Enzymes
X-ray crystallography
Medam @ Hamdan, Siti Hajar
Structural determination of improved methanol-tolerant mutant from Geobacillus zalihae T1 lipase by x-ray crystallography
description Lipases are versatile enzymes that have been altered through various modification methods to improve their enzymatic properties to meet biotechnology industry requirement. Since decades ago, lipases from many sources have been study widely as potential biocatalyst to assist synthesis of biodiesel. Some of them have been altered via protein engineering approach to enhance their enzymatic performance and stability. The thermostable T1 lipase from Geobacillus zalihae can also be a great biocatalyst candidate in biodiesel production. However, inactivation of T1 lipase when the enzyme is surrounded by high concentration of methanol solvent is limiting its uses in industrial applications. Since introduction of non-bonded interactions hardly improved their stability of T1 lipase in methanol, the introduction of disulphide bond could be the best proposition to retain protein conformation and the enzyme stability in the presence of methanol. Hence, current study aims to engineer a methanoltolerant lipase by site-directed mutagenesis and divulge the interaction that stabilizes the mutant by X-ray crystallography. The preliminary study on enzyme stability was conducted by using online software ERIS, FoldX and MAESTRO. The stability of the mutant 2DC lipase was tested virtually and molecular dynamic simulation was performed in water and methanol solvent. Experimentally, the purified protein of mutant 2DC lipase was used to screen protein crystal for diffraction to elucidate and validate the mutant’s structure. It showed that the substitution of amino acid S2 and A384 with cysteine could enhance the stability of the enzyme by promoting the formation of disulphide bond to tighten the both terminal ends of the protein structure. The substitution of amino acid cysteine showed the changes on the active site distance (S113, D317, and H358), however, it was not affected the lipase activity and folding of protein structure. The 2DC mutant was successfully constructed and cloned into pET32-b and transformed into Origami B (DE3) expression host. The expression and purification using Ni2+-Sepharose affinity chromatography and gel filtration chromatography S-200 of the protein yielding 4.0 mg/ml mutant 2DC lipase suitable for protein crystallization. The mutant 2DC lipase was crystallized after 24-hour incubation at 20°C and diffracted by X-ray crystallography for deeper evaluation in term of stability and rigidity. The crystal was diffracted at 2.04 Å using in-house X-ray beam and the crystal belongs to monoclinic space group C2, with unit cell parameter of a = 118.17, b = 81.5, c = 100.05. Details information on structural elucidation of the mutant 2DC lipase has disclosed the changes within the mutant structure which associated with the alteration of enzyme activity and stability posed by the mutant. The increased in rigidity of the structure as well as changes of interaction within the catalytic region of the mutant 2DC lipase were suggested to be the factor influenced its enzymatic activity, stability and tolerance towards methanol. Hence, this newly improved mutant 2DC lipase could be the next potential biocatalyst in biodiesel production industry.
format Thesis
author Medam @ Hamdan, Siti Hajar
author_facet Medam @ Hamdan, Siti Hajar
author_sort Medam @ Hamdan, Siti Hajar
title Structural determination of improved methanol-tolerant mutant from Geobacillus zalihae T1 lipase by x-ray crystallography
title_short Structural determination of improved methanol-tolerant mutant from Geobacillus zalihae T1 lipase by x-ray crystallography
title_full Structural determination of improved methanol-tolerant mutant from Geobacillus zalihae T1 lipase by x-ray crystallography
title_fullStr Structural determination of improved methanol-tolerant mutant from Geobacillus zalihae T1 lipase by x-ray crystallography
title_full_unstemmed Structural determination of improved methanol-tolerant mutant from Geobacillus zalihae T1 lipase by x-ray crystallography
title_sort structural determination of improved methanol-tolerant mutant from geobacillus zalihae t1 lipase by x-ray crystallography
publishDate 2022
url http://psasir.upm.edu.my/id/eprint/113000/1/113000.pdf
http://psasir.upm.edu.my/id/eprint/113000/
_version_ 1814054779782955008

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