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Heterologous Expression Of Recombinant Cellulase In Escherichia Coli Rosetta (De3) And Bl21 (De3)

The heterologous expression of cellulase gene from Aspergillus sp. in E.coli strains of Rosetta (DE3) and BL2 l (DE3) has been studied to compare the recombinant protein production and to observe their activity, efficiency and production rate of recombinant cellulase. In previous study, an improv...

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Main Author: Casandra, Kana Brooke
Format: Final Year Project Report
Language:English
English
Published: Universiti Malaysia Sarawak, (UNIMAS) 2018
Subjects:
Q Science (General)
Online Access:http://ir.unimas.my/id/eprint/35379/1/Heterologous%20Expression%20Of%20Recombinant%20Cellulase%20In%20Escherichia%20Coli%20Rosetta%20%28De3%29%20And%20Bl21%20%28De3%29%2824pgs%29.pdf
http://ir.unimas.my/id/eprint/35379/4/Heterologous%20Expression..ft.pdf
http://ir.unimas.my/id/eprint/35379/
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spelling my.unimas.ir.353792023-03-02T08:43:15Z http://ir.unimas.my/id/eprint/35379/ Heterologous Expression Of Recombinant Cellulase In Escherichia Coli Rosetta (De3) And Bl21 (De3) Casandra, Kana Brooke Q Science (General) The heterologous expression of cellulase gene from Aspergillus sp. in E.coli strains of Rosetta (DE3) and BL2 l (DE3) has been studied to compare the recombinant protein production and to observe their activity, efficiency and production rate of recombinant cellulase. In previous study, an improved protein quality has been detected by using Rosetta, therefore further works need to be carried out to compare its protein production with BL2 l. The pFT AG-vector with the recombinant cellulase was used for expression studies and inserted into both Rosetta and BL2 l. Screening of cellullolyctic organism has failed to reveal the activity of recombinant cellulase as there is no growth detected on the media, as well as no formation of halo zone. Other than detection using the formation of halo zone, Bradford Assay and DNS assay was conducted to determine the cellulase activity of the bacterial in liquid medium. Recombinant cellulase from Rosetta was shown to have higher cellulase activity when the protein concentration was calculated using the standard graph. It was due to the fact that Rosetta has rare codons implemented inside them in order to yield higher protein production and better protein purity Universiti Malaysia Sarawak, (UNIMAS) 2018 Final Year Project Report NonPeerReviewed text en http://ir.unimas.my/id/eprint/35379/1/Heterologous%20Expression%20Of%20Recombinant%20Cellulase%20In%20Escherichia%20Coli%20Rosetta%20%28De3%29%20And%20Bl21%20%28De3%29%2824pgs%29.pdf text en http://ir.unimas.my/id/eprint/35379/4/Heterologous%20Expression..ft.pdf Casandra, Kana Brooke (2018) Heterologous Expression Of Recombinant Cellulase In Escherichia Coli Rosetta (De3) And Bl21 (De3). [Final Year Project Report] (Unpublished)
institution Universiti Malaysia Sarawak
building Centre for Academic Information Services (CAIS)
collection Institutional Repository
continent Asia
country Malaysia
content_provider Universiti Malaysia Sarawak
content_source UNIMAS Institutional Repository
url_provider http://ir.unimas.my/
language English
English
topic Q Science (General)
spellingShingle Q Science (General)
Casandra, Kana Brooke
Heterologous Expression Of Recombinant Cellulase In Escherichia Coli Rosetta (De3) And Bl21 (De3)
description The heterologous expression of cellulase gene from Aspergillus sp. in E.coli strains of Rosetta (DE3) and BL2 l (DE3) has been studied to compare the recombinant protein production and to observe their activity, efficiency and production rate of recombinant cellulase. In previous study, an improved protein quality has been detected by using Rosetta, therefore further works need to be carried out to compare its protein production with BL2 l. The pFT AG-vector with the recombinant cellulase was used for expression studies and inserted into both Rosetta and BL2 l. Screening of cellullolyctic organism has failed to reveal the activity of recombinant cellulase as there is no growth detected on the media, as well as no formation of halo zone. Other than detection using the formation of halo zone, Bradford Assay and DNS assay was conducted to determine the cellulase activity of the bacterial in liquid medium. Recombinant cellulase from Rosetta was shown to have higher cellulase activity when the protein concentration was calculated using the standard graph. It was due to the fact that Rosetta has rare codons implemented inside them in order to yield higher protein production and better protein purity
format Final Year Project Report
author Casandra, Kana Brooke
author_facet Casandra, Kana Brooke
author_sort Casandra, Kana Brooke
title Heterologous Expression Of Recombinant Cellulase In Escherichia Coli Rosetta (De3) And Bl21 (De3)
title_short Heterologous Expression Of Recombinant Cellulase In Escherichia Coli Rosetta (De3) And Bl21 (De3)
title_full Heterologous Expression Of Recombinant Cellulase In Escherichia Coli Rosetta (De3) And Bl21 (De3)
title_fullStr Heterologous Expression Of Recombinant Cellulase In Escherichia Coli Rosetta (De3) And Bl21 (De3)
title_full_unstemmed Heterologous Expression Of Recombinant Cellulase In Escherichia Coli Rosetta (De3) And Bl21 (De3)
title_sort heterologous expression of recombinant cellulase in escherichia coli rosetta (de3) and bl21 (de3)
publisher Universiti Malaysia Sarawak, (UNIMAS)
publishDate 2018
url http://ir.unimas.my/id/eprint/35379/1/Heterologous%20Expression%20Of%20Recombinant%20Cellulase%20In%20Escherichia%20Coli%20Rosetta%20%28De3%29%20And%20Bl21%20%28De3%29%2824pgs%29.pdf
http://ir.unimas.my/id/eprint/35379/4/Heterologous%20Expression..ft.pdf
http://ir.unimas.my/id/eprint/35379/
_version_ 1759693322632298496
score 13.15806

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