Proof of concept - Fungi
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Filamentous Fungi
Fungi are a diverse group of organisms, whose biological activities affect our daily life in many ways. The filamentous fungi are in particular of great importance in production of medicine, in the industry, in agriculture, and in basic biological research. Some of the filamentous fungal species are pathogenic to humans, whereas others have great value in the production of antibiotics such as penicillin. The fungi are therefore importance for industrial as well as medical production. Growth of filamentous fungiThe vegetative growth of filamentous fungi start with the germination of a spore when the conditions are right . The spore germination leads to formation of hyphae (1). A fungal hypha is a long tubular modular structure composed of individual cells (2). Hyphae extend only at their tips and are typically divided into individual cellular compartments by the formation of septa (3).
Filamentous fungi grow by the polar extension of hyphae and multiply by branching (4). The branched hyphae forms a network of interconnected cells called a mycelium (1). The mycelium forms a radially symmetric colony that expands over large area until growth is limited by for example lack of nutrients (1,5). The fungal mycelium appears to be a formless collection of corresponding vegetative cells. However, the various cells within the mycelium interact to form an ordered network with different hyphae or cells playing distinct roles in the acquirement of nutrients from the environment and development (1). Aspergillus nidulans
The filamentous fungus Aspergillus nidulans is a widely recognised model organism (3). A. nidulans possesses today, in contrast to most other aspergilla, a well characterized sexual cycle and a well-developed genetics system (6). Furthermore, in A.nidulans the parasexual cycle has been extensively utilized. Parasexual genetic involves examination of recombination in the absence of sexual reproduction. Gene targetingAccurate manipulation of genes is a key approach in fungal molecular biology (9). The method of gene targeting facilitates precise genome manipulations which are called site directed alterations. They are performed by use of deletions, replacements and insertion in the target locus. Gene targeting is achieved by transforming fungi with a suitable linear DNA fragment that contains sequences that are identical to the target site in the genome, see figure below. Different DNA fragments are constructed depending on deletion, replacement or insertion. The fungi can integrates linear DNA fragment in its genome by using its repair system of DNA double stranded breaks.
Two mechanisms of DNA double strand break repair ensure that the introduced piece of DNA is pasted into the fungal genome, to be replicated stably; Homologous Recombination and Non Homologous End Joining, also called illegitimate recombination (9). Homologous recombination involves interaction between homologous sequences, whereas Non Homologous End Joining involves ligation of the strand ends independently of DNA homology (10). Precise genome manipulation can often be tedious and time-consuming, because fungi appear to favour Non Homologous End Joining over Homologous recombination resulting in low gene targeting efficiencies (9). Proof of concept
Several separate plasmid was constructed by use of the Plug 'n' Play assembly system to verify the systems function in filamentous fungi. To perform a successful transformation in fungi the backbone plasmid for the fungal devices BBa_K678046 have two NotI restriction sites flanking the device. Hereby, the device can be cut and a linearised DNA fragment can be transformated into the fungi. The devices for proof of concept in fungi are not design to be inserted at a specific site at the fungal genome. Therefore, a fungal strain with intact pathway for non homologous recombination was used. Therefore, the device can integrate at any site in the fungi and thereby also at site of essential genes.
We succeeded in proving that the Plug 'n' Play assembly system is easily applied for constructing fungal vectors. Transformation and expression of the fluorescence proteins GFP and RFP was successfully conducted in A. nidulans, not localized to any compartment.Furthermore, expression of fluorescence proteins GFP and RFP in A. nidulans localized to the nucleus and the peroxiomes succeeded. However, the transformation of the fungi with the mitochondrial targeting signal did not succeed.
The results of the created reporter system for fungi are displayed below. Device BBa_K678060Observed is green fluorescence spread evenly in the hyphae, which correlate with what was expected for the device BBa_K678060 that holds the gene for green fluorescence protein GFP with no specific targeting signal.
The pJEJAM 12 plasmid constructed holding device BBa_K678060, which are cut at the two NotI site before transformation, ensure linearised DNA fragment for optimal result.
Device BBa_K678061Green fluorescence is observed and are spread in the hyphae and in clear spots. The occurrence of clear spots and compared to the results from device BBa_K678060, correlate with what expected for the device BBa_K678061 that holds the gene for green fluorescence protein GFP with the targeting signal for the peroxiomes. However, we cannot conclude that the signal is accumulated in the peroxisomes, since they are not dyed. Though, it can be concluded that the GFP signal is targeting to a specific place and accumulated somewhere in the fungi compared to the results from device BBa_K678060.
The pJEJAM 13 plasmid constructed holding device BBa_K678061, which are cut at the two NotI site before transformation, ensure linearised DNA fragment for optimal result.
Device BBa_K678062Observed is red fluorescence spread evenly in the hyphae, which correlate with what expected for the device BBa_K678062 that holds the gene for red fluorescence protein RFP with no specific targeting signal.
The pJEJAM 14 plasmid constructed holding device BBa_K678062, which are cut at the two NotI site before transformation, ensure linearised DNA fragment for optimal result.
Device BBa_K678063Observed is red fluorescence spread in clear spots. The occurrence of clear spots and compared to the results from device BBa_K678062, correlate with what expected for the device BBa_K678063 that holds the gene for red fluorescence protein RFP with the targeting signal for the nucleus. However, we cannot conclude that the signal is accumulated in the nucleus, since they are not dyed. Though, it can be concluded that the RFP signal is targeting to a specific place and accumulated somewhere in the fungi compared to the results from device BBa_K678062.
The pJEJAM 15 plasmid constructed holding device BBa_K678063, which are cut at the two NotI site before transformation, ensure linearised DNA fragment for optimal result.
Control strainThe control strain shows no background or auto-fluorescence.
References
[1] Adams, T.H., Wieser, J.K. & Yu, J.-H., 1998. Asexual Sporulation in Aspergilus nidulans. Microbiology and Molecular Biology Reveiws, vol. 62, no. 1, pp.35-54.
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