Aspergillus niger

From MicrobeWiki, the student-edited microbiology resource

A Microbial Biorealm page on the genus Aspergillus niger

Classification

Higher order taxa

Cellular organisms; Eukaryota; Fungi/Metazoa group; Fungi; Dikarya; Ascomycota; Pezizomycotina; Eurotiomycetes; Eurotiomycetidae; Eurotiales; Trichocomaceae; mitosporic Trichocomaceae; Aspergillus

Species

NCBI: Taxonomy

Aspergillus niger

Description and significance

Aspergillus niger is a haploid filamentous fungi and is a very essential microorganism in the field of biology. In addition to producing extracellular enzymes and citric acid, A. niger is used for waste management and biotransformations. The fungi is most commonly found in mesophilic environments such as decaying vegetation or soil and plants. (2)

Genome sequencing of A. niger is important because of its involvement in producing citric acid as well as industrial enzymes, such as amylases, proteases, and lipases. The use of these enzymes are essential because of its importance for transformation to food enzymes. Other properties of this species include pathogens that cause the spoilage of food and production of secondary metabolites, such as aflatoxin, that are toxic. Metabolite production, involvement in food spoilage, and simply being a pathogen creates a great economic impact on the U.S. (roughly $45 billion on the U.S. economy alone). Understanding this economic importance as well as the effects it makes on the environment makes the genome sequencing of A. niger essential to biological applications.(4, 5)

A. niger was isolated from the plant Welwitschia mirabilis in Namibia and Angola, a plant estimated to be about 3000 years old. A. niger is easily isolated from common thing such as dust, paint, and soil. Commonly in labs, A. niger is isolated via chemostat cultures which can test positively or negatively for the fungi. (3, 6)

Genome structure

A. niger have a total genome size that ranges from 35.5 to 38.5 Mb and is composed of about 13,000 genes. Of these genes, about 8000 to 8500 genes have functional assignments. In addition, about 14,000 open reading frames (ORF) were identified in the genome which could potentially encode a protein. The DNA sequence of A. niger consists of approximately 33.9 million base pairs. The possible function of 6500 genes could be established which is only about 45% of its total gene count.(7)

Electrophoretic karyotyping of A. niger allows the visualization of chromosomes separated into four separate bands. The chromosomal bands range from 3.5 to 6.6 Mb. The karyotype sequence that was obtained could be arranged into 19 separate supercontigs that correspond to eight linear chromosomes.(7)

Treating A. niger with recombinant DNA allows spheroplasts to take up some recombinant DNA. Recombinant DNA has the properties of being both linear and circular and is also used as a selectable marker (since A. niger does not have a programmed selectable marker) which has an antibiotic resistance to transformants. The selectable marker is known as the ornithine carbamoyl transferase gene (Arg B. sup +) and encodes a product that can be assayed. (8)

The recombinant DNA contains a replicon which allows for replication in a bacterial host. The recombinant DNA consists of a plasmid vectors pDG1 (ATCC 53005) and pDG3 (ATCC 53006). Transformation of these vectors includes removing the cell wall enzymatically, adding exogenous DNA to the spheroplasts, and incubating so the spheroplasts take up the DNA. Once this process is complete, isolation of the A. niger transformant is possible.(8)

Cell structure and metabolism

A. niger produce colonies that are composed of white or yellow felt that is covered by dark asexually produced fungal spores. Mycelial, or threadlike, hyphae are divided by a septum and transparent. Conidiophores (asexually produced fungal spores) of A. niger usually range from 900-1600 µm in length and contain globose (globular) vesicles ranging from 40-60 µm in diameter. Each globose vesicle is completely covered with biseriate phialides which are projections from the conidiophore of A. niger. These phialides come out from brown metulae, which is the site where a conidiogenous cell is created. The phialides go through a process of blastic basipetal conidiogenesis to create globose mitospores, which have a diameter that ranges from 3 to 5 µm. (7)

One of the most common ways that A. niger gains energy is through bioleaching. Bioleaching is the process of extracting metals from ores via the use of bacteria. A. niger gains its energy by breaking down the minerals into its most basic element. This fungi specifically is able to break down copper, tin, aluminum, nickel, and lead, and with this energy is able to produce oxalic acid, gluconic acid, and citric acid. (9)

Different reactions and pathways are used whenever A. niger consumes a substrate or forms a metabolic product. Chitin, for example, makes up the cell wall of A. niger, however the only enzymatic steps that are used to create chitin are those catalyzed by glutamine-fructose-6-phosphate transaminase as well as chitin synthase. (10)

One of the most important products that A. niger produces is citric acid. Under conditions of citric acid accumulation, the metabolism of A. niger is slightly altered. In normal conditions metabolism of the fungi progresses at a linear rate. In this linearly progressive state, production of citric acid is high, however there is still an opportunity for changes which can lead to a five fold increase in basal rate synthesis. Again, this value can be further increased with a doubling in enzyme concentration. Doubling the concentration allows at least a 12 fold increase in citric acid production and a maximum of a 50 fold increase when enzyme concentration is 10 times its normal value. Under optimal conditions, at least 13 enzymes need to be altered in order to obtain a maximum in citric acid production.(11)

Ecology and Pathology

A. niger is usually found in common mesophilic environments such as soil, plants, and enclosed air environments. A. niger is not only a xerophilic fungi (mold that doesn’t require free water for growth, can grow in humid environments), but is also a thermotolerant organism (capable of growing at high temperatures). Because of this property, the filamentous fungi exhibits a high tolerance to freezing temperatures. (2)

A. niger is relatively harmless compared to other filamentous fungi. Despite this fact, there have been some medical cases that have been accounted for, such as lung infections or ear infections in patients that have an weakened immune system, or an immune system that has been impaired by a disease or medical treatment. In the case of ear infections, A. niger invades the outer ear canal which can cause damage to the skin it came in contact with. (2, 4)

This species of filamentous fungi produces several secondary metabolites, one of the most important being ochratoxin A. Ochratoxin A is an abundant food-contaminating mycotoxin. Human contact with this toxin usually occurs through consumption of food which has not been stored and taken care of appropriately. Nevertheless, studies have shown that less that 10% of the A. niger strains were tested positive for ochratoxin A under conditions that were favorable. (2)

The productioin of ochratoxin A from A. niger, is liable to cause immunotoxcitiy in animals. The effects on animals include a decrease in antibody responses, a size reduction in immune organs, and an alteration in the production of cytokine which are proteins and peptides specifically used in signaling. Food that has been contaminated by A. niger’s toxic metabolite has had a major affect on the poultry industry. Different animals, such as chicken, turkey, and ducks, are very prone to ochratoxin. (2, 4)

Application to Biotechnology

A. niger has been a very important microbe used in the field of biotechnology. Many of the enzymes produced by A. niger, such as citric acid, amylases, lipases, cellulases, xylanases and proteases, are considered GRAS (generally recognized as safe) by the United States Food and Drug Administration and is excused from the Federal Food, Drug, and Cosmetic Act food additive tolerance requirements. Even though it is considered GRAS, A. niger still must be treated safely and with care. (2, 6)

(For further information on citric acid production, see Cell Structure and Metabolism)

A. niger has also been used for waste treatment and chemical modifications known as biotransformations. In the past 20 years, A. niger has been used as a host for transformation to food enzymes. However, it is still important to treat this fungi very carefully to avoid formation of spore dust which can cause illness (see pathology). However, checking for ochratoxin A, a mycotoxin, can reduce any risks and will yield A. niger as a safe organism.(2, 6)

Current Research

Phytases have the property of catalyzing phosphate hydrolysis from phytate. Phytate is used for absorption by animals. In normal circumstances, A. niger PhyB has an optimal catalytic activity at an average pH of 2.5. This poses a problem since the pH of animal’s stomachs range from 3.0 to 3.5. In order to shift the pH optimum of A. niger PhyB, modification of the substrate specificity site must be performed. Mutants (E272K, E272Q) were used which affects the substrate specificity site, and results showed that mutant E272K shifted the pH optimum from 2.5 to 3.2. From this, it is possible to change the pH optimum to mirror that of the stomach which will result in a greater substrate attraction. (12)

One of the top waste materials of fish processing industries is fish scale. A. niger plays an important role because fish scale is processed by protease from mutant Aspergillus niger AB100. With fish scale present, protease production from A. niger AB100 was improved a great deal. Testing of the AB100 in different environments was necessary to see what environment would be optimal for protease production. Results show that AB100 in contact with soy bean meal produces the greatest protease production. Conditions at which production was maximal included a pH at 7 with a temperature of 50°C. Activity in pH 5 to pH 9 resulted in 60% protease production, and at a temperature of 30°C, protease production was stable as opposed to active. (13)

Thigmotropism is topographical sensing and this is an important factor of growth in A. niger. Thigmotropism is essential to help provide growth for the hyphal tip. Past studies have shown that strain, caused by nutrient shortage, causes a structural transformation in the hyphal tip that stimulates a topographical sensing response in A. niger. Since A. niger doesn’t usually exhibit thigmotropism under a typical environment, experiments were conducted in order to find variables which induce thigmotropism. Results show that topographical sensing is directly related to how much nutrients are available. In addition, the study also shows that thigmotropism is caused by a stress reaction in the fungal hyphae where the tip flattens. (14)

References

(1) NCBI: Aspergillus niger, Accessed August 23, 2007, <http://www.ncbi.nlm.nih.gov/Taxonomy/Browser/wwwtax.cgi?mode=Info&id=380704&lvl=3&p=mapview&p=has_linkout&p=blast_url&p=genome_blast&lin=f&keep=1&srchmode=1&unlock>

(2) Schuster, E., Dunn-Coleman, N., Frisvad, J., van Dijck, P. “On the safety of Aspergillus niger – a review”. Applied Microbiology and Biotechnology. 2002. Volume 59. p. 426-435.

(3) Pekarek, E., Jacobson, K., Donovan, A. “High Levels of Genetic Variation Exist in Aspergillus niger Populations Infecting Welwitschia mirabilis Hook”. Journal of Heredity. 2006. Volume 97. p. 270-278.

(4) May, G., Adams, T. “The Importance of Fungi to Man”. Genome Research. 1997. Volume 7. p. 1041-1044.

(5) Takahashi, K., Inoue, H., Sakai, K., Kohama, T., Kitahara, S., Takishima, K., Tanji, M., Athauda, S., Takahashi, T., Akanuma, H. “The primary structure of Aspergillus niger acid proteinase A”. The Journal of Biological Chemistry. 1991. Volume 266. p. 19480-19483.

(6) Van de Vondervoort, P., Poulsen, B., Ruijter, G., Schuleit, T., Visser, J., Iversen, J. “Isolation of a fluffy mutant of Aspergillus niger from chemostat culture and its potential use as a morphological stable host for protein production”. Biotechnology and Bioengineering. 2004. Volume 86. p. 301-307.

(7) Debets, A., Holub, E., Swart, K., van den Broek, H., Bos, C. “An electrophoretic karyotype of Aspergillus niger”. Molecular and General Genetics. 1990. Volume 224. p. 1432-1874.

(8) Mohr, G., Wilmanska, D., Esser, K. “Analysis of Aspergillus niger transformants for single site integration and vector recombination”. Applied Microbiology and Biotechnology. 1989. Volume 32. p. 160-166.

(9) Santhiya, D., Ting, Y. “Bioleaching of spent refinery processing catalyst using Aspergillus niger with high-yield oxalic acid”. Journal of Biotechnology. 2005. Volume 116. p. 171-184.

(10) David, H., Akesson, M., Nielsen, J. “Reconstruction of the central carbon metabolism of Aspergillus niger”. European Journal of Biochemistry. 2003. Volume 270. p. 4243-4253.

(11) Alvarez-Vasquez, F., Gonzalez-Alcon, C., Torres, N. “Metabolism of citric acid production by Aspergillus niger: Model definition, steady-state analysis and constrained optimization of citric acid production rate”. Biotechnology and Bioengineering. 2000. Volume 70. p. 82-108.

(12) Weaver, J., Mullaney, E., Lei, X. “Altering the substrate specificity site of Aspergillus niger PhyB shifts the pH optimum to pH 3.2”. Applied Microbiology and Biotechnology. 2007. Volume 76. p. 117-122

(13) Basu, B., Banik, A., Das, M. “Production and characterization of extracellular protease of mutant Aspergillus niger AB100 grown on fish scale”. World Journal of Microbiology and Biotechnology. 2007.

(14) Bowen, A., Davidson, F., Keatch, R., Gadd, G. “Effect of nutrient availability on hyphal maturation and topographical sensing in Aspergillus niger”. Mycoscience. 2007. Volume 48. p. 145-151.


Edited by Kyle Choi student of Rachel Larsen