Engineering biofilm matrix for efficient biofilm-mediated contaminant removal
The naturally sorptive nature of biofilm matrix is an attractive feature to be exploited for environmental application. The objective of this thesis work is to engineer biofilm matrix into an enhanced biosorbent for efficient biofilm-mediated contaminant removal. Shewanella oneidensis was used...
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Nanyang Technological University
2021
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Engineering::Bioengineering Science::Biological sciences::Microbiology::Bacteria Science::Biological sciences::Molecular biology |
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Engineering::Bioengineering Science::Biological sciences::Microbiology::Bacteria Science::Biological sciences::Molecular biology Zaiden, Norazean Engineering biofilm matrix for efficient biofilm-mediated contaminant removal |
| description |
The naturally sorptive nature of biofilm matrix is an attractive feature to be exploited for
environmental application. The objective of this thesis work is to engineer biofilm matrix into
an enhanced biosorbent for efficient biofilm-mediated contaminant removal. Shewanella
oneidensis was used as an environmentally relevant model organism for biofilm matrix
modification through manipulating an abundant matrix-associated protein, BpfA. Arsenic (As)
was the contaminant in focus to demonstrate the aimed enhanced sorption by the engineered
biofilm.
To understand the role of BpfA in the interaction between S. oneidensis and As, comparisons
were performed on the global transcriptomics from the RNA-sequencing of the wild-type
(WT) and the BpfA-lacking mutant bpfA. When treated with As, both the WT and the
bpfA were shown to upregulate the ars-detoxification system for As tolerance, and the
master regulator of metabolic processes, TyrR. Energy-consuming metabolic enzymes and
low energy efficient metabolic pathways were downregulated in both. The lack of BpfA
resulted in expression loss of genes that are primarily important for managing oxidative stress,
protein synthesis and their quality assessment, amino acid and phospholipid biosynthesis,
uptake of sulfate and exports of xenobiotics. These losses were observed to be compensated
with the expression of megaplasmid-borne genes promoting cellular preservation by
regulating the cellular metal content and defense, genetic information, and flux of exogenous
genetic materials.
With the aim to display As-binding domains in the S. oneidensis biofilm matrix, the
chromosomal bpfA was genetically fused to arsR from E. coli, which encodes for a well-characterized As binding protein. The recombinant exhibited poor aggregation under rapid
agitation but showed competency in biofilm formation under hydrodynamic conditions.
Sorption of As by the engineered biofilms was quantified using packed-bed biofilm reactors
and the results showed ~2-fold higher sorption by the recombinant biofilms than the WT
biofilms. To overcome the limitation of expressing BpfA-ArsR through the only 1 copy
chromosomal bpfA in S. oneidensis, an expression of a higher copy number of bpfA was
attempted using vector systems. Due to its high repeats content and to accommodate its
insertion into a vector system, the bpfA gene was truncated to encode domains deemed
necessary for biofilm formation. Biofilm formation assay revealed the necessity of the RTX
domain. Constitutive and high induction of BpfA truncates expression resulted in low amounts of biofilm formation. In contrast, substantial biofilm formed when the BpfA
truncates were expressed in an IPTG-inducible vector system. This then allowed a further
engineering of it to co-express ArsR, As-specific binding module, at its C-terminal end to be
displayed as a component in the biofilm matrix for As sorption. When compared to WT, the
As sorption by the biofilms of the vector-expressed BpfA-ArsR recombinants exhibited 3.6-
fold more, while the biofilms of the recombinant expressing BpfA-ArsR in the chromosome
exhibited 2.4-fold more. Therefore, implicating that vector-expressed BpfA-ArsR can
increase As sorption through higher expression of BpfA-ArsR. Taken together, this thesis
work reports the practicality of engineering biofilm matrix into a sustainable biological tool
for environmental applications. Modifying an extracellular polymeric substance in biofilms
can enhance its sorptive nature as shown in this thesis work and may also serve as a strategy
to create other functional biofilms. |
| author2 |
Cao Bin |
| author_facet |
Cao Bin Zaiden, Norazean |
| format |
Thesis-Doctor of Philosophy |
| author |
Zaiden, Norazean |
| author_sort |
Zaiden, Norazean |
| title |
Engineering biofilm matrix for efficient biofilm-mediated contaminant removal |
| title_short |
Engineering biofilm matrix for efficient biofilm-mediated contaminant removal |
| title_full |
Engineering biofilm matrix for efficient biofilm-mediated contaminant removal |
| title_fullStr |
Engineering biofilm matrix for efficient biofilm-mediated contaminant removal |
| title_full_unstemmed |
Engineering biofilm matrix for efficient biofilm-mediated contaminant removal |
| title_sort |
engineering biofilm matrix for efficient biofilm-mediated contaminant removal |
| publisher |
Nanyang Technological University |
| publishDate |
2021 |
| url |
https://hdl.handle.net/10356/154444 |
| _version_ |
1759854670413561856 |
| spelling |
sg-ntu-dr.10356-1544442023-03-05T16:34:00Z Engineering biofilm matrix for efficient biofilm-mediated contaminant removal Zaiden, Norazean Cao Bin Interdisciplinary Graduate School (IGS) Singapore Centre for Environmental Life Sciences and Engineering (SCELSE) BinCao@ntu.edu.sg Engineering::Bioengineering Science::Biological sciences::Microbiology::Bacteria Science::Biological sciences::Molecular biology The naturally sorptive nature of biofilm matrix is an attractive feature to be exploited for environmental application. The objective of this thesis work is to engineer biofilm matrix into an enhanced biosorbent for efficient biofilm-mediated contaminant removal. Shewanella oneidensis was used as an environmentally relevant model organism for biofilm matrix modification through manipulating an abundant matrix-associated protein, BpfA. Arsenic (As) was the contaminant in focus to demonstrate the aimed enhanced sorption by the engineered biofilm. To understand the role of BpfA in the interaction between S. oneidensis and As, comparisons were performed on the global transcriptomics from the RNA-sequencing of the wild-type (WT) and the BpfA-lacking mutant bpfA. When treated with As, both the WT and the bpfA were shown to upregulate the ars-detoxification system for As tolerance, and the master regulator of metabolic processes, TyrR. Energy-consuming metabolic enzymes and low energy efficient metabolic pathways were downregulated in both. The lack of BpfA resulted in expression loss of genes that are primarily important for managing oxidative stress, protein synthesis and their quality assessment, amino acid and phospholipid biosynthesis, uptake of sulfate and exports of xenobiotics. These losses were observed to be compensated with the expression of megaplasmid-borne genes promoting cellular preservation by regulating the cellular metal content and defense, genetic information, and flux of exogenous genetic materials. With the aim to display As-binding domains in the S. oneidensis biofilm matrix, the chromosomal bpfA was genetically fused to arsR from E. coli, which encodes for a well-characterized As binding protein. The recombinant exhibited poor aggregation under rapid agitation but showed competency in biofilm formation under hydrodynamic conditions. Sorption of As by the engineered biofilms was quantified using packed-bed biofilm reactors and the results showed ~2-fold higher sorption by the recombinant biofilms than the WT biofilms. To overcome the limitation of expressing BpfA-ArsR through the only 1 copy chromosomal bpfA in S. oneidensis, an expression of a higher copy number of bpfA was attempted using vector systems. Due to its high repeats content and to accommodate its insertion into a vector system, the bpfA gene was truncated to encode domains deemed necessary for biofilm formation. Biofilm formation assay revealed the necessity of the RTX domain. Constitutive and high induction of BpfA truncates expression resulted in low amounts of biofilm formation. In contrast, substantial biofilm formed when the BpfA truncates were expressed in an IPTG-inducible vector system. This then allowed a further engineering of it to co-express ArsR, As-specific binding module, at its C-terminal end to be displayed as a component in the biofilm matrix for As sorption. When compared to WT, the As sorption by the biofilms of the vector-expressed BpfA-ArsR recombinants exhibited 3.6- fold more, while the biofilms of the recombinant expressing BpfA-ArsR in the chromosome exhibited 2.4-fold more. Therefore, implicating that vector-expressed BpfA-ArsR can increase As sorption through higher expression of BpfA-ArsR. Taken together, this thesis work reports the practicality of engineering biofilm matrix into a sustainable biological tool for environmental applications. Modifying an extracellular polymeric substance in biofilms can enhance its sorptive nature as shown in this thesis work and may also serve as a strategy to create other functional biofilms. Doctor of Philosophy 2021-12-27T12:27:46Z 2021-12-27T12:27:46Z 2021 Thesis-Doctor of Philosophy Zaiden, N. (2021). Engineering biofilm matrix for efficient biofilm-mediated contaminant removal. Doctoral thesis, Nanyang Technological University, Singapore. https://hdl.handle.net/10356/154444 https://hdl.handle.net/10356/154444 10.32657/10356/154444 en This work is licensed under a Creative Commons Attribution-NonCommercial 4.0 International License (CC BY-NC 4.0). application/pdf Nanyang Technological University |