Mutation breeding of Aspergillus niger by atmospheric room temperature plasma to enhance phosphorus solubilization ability

Background Phosphorus (P) is abundant in soils, including organic and inorganic forms. Nevertheless, most of P compounds cannot be absorbed and used by plants. Aspergillus niger v. Tiegh is a strain that can efficiently degrade P compounds in soils. Methods In this study, A. niger xj strain was mutated using Atmospheric Room Temperature Plasma (ARTP) technology and the strains were screened by Mo-Sb Colorimetry with strong P-solubilizing abilities. Results Compared with the A. niger xj strain, setting the treatment time of mutagenesis to 120 s, four positive mutant strains marked as xj 90–32, xj120–12, xj120–31, and xj180–22 had higher P-solubilizing rates by 50.3%, 57.5%, 55.9%, and 61.4%, respectively. Among them, the xj120–12 is a highly efficient P solubilizing and growth-promoting strain with good application prospects. The growth characteristics such as plant height, root length, and dry and fresh biomass of peanut (Arachis hypogaea L.) increased by 33.5%, 43.8%, 43.4%, and 33.6%, respectively. Besides available P, the chlorophyll and soluble protein contents also vary degrees of increase in the P-solubilizing mutant strains. Conclusions The results showed that the ARTP mutagenesis technology can improve the P solubilization abilities of the A. niger mutant strains and make the biomass of peanut plants was enhanced of mutant strains.


INTRODUCTION
Phosphorus (P) is the second essential macronutrient for plant growth and development. Although P only accounts for 0.2% of plant dry weight, low P availability can generate a strong limit in plant growth and crop yield (Sharma et al., 2013). The natural reserve of soluble P fractions is much lower than expected, which may just have a range of doses Mutagenesis tools, including chemical mutagens, physical or biological approaches, are used to increase mutation rate and accelerate the subsequent evolutionary process to obtain mutant strains with desirable phenotypes (Huang et al., 2021). Among them, Atmospheric Room Temperature Plasma (ARTP) mutagenesis technology caused more serious DNA damage and a higher mutation rate among all the mutagenesis methods . ARTP is a novel type of atmospheric pressure non-equilibrium discharge plasma source, which relies on a uniform distribution of highly concentrated neutral active particles to alter microbial genetic traits and directly modify the molecular structure at a nucleotide level (Zong et al., 2012). It has wide applications and high efficiency of mutation diversity and offers good safety and ease-of-use (Zhang et al., 2014). ARTP mutagenic technology has been successful in obtaining strains with desirable characteristics among bacteria, fungi, and microalgae (Zhang et al., 2019a(Zhang et al., , 2019b. Zong et al. (2012) used ARTP technology to generate mutations in Streptomyces albulus, and the spores concentration was 10 6 CFU mL -1 , which the positive mutation rates can reach a level as high as up to 26.0%. S. albulus A-29 exhibited the highest ε-Poly-L-lysine productivity, which was four times higher than that of the wild strain in the same culture condition. Song et al. (2017) revealed that, compared with the original strain, the lipid productivity of Chlorella pyrenoidosa was nearly improved over 16% by ARTP. The above examples illustrate that ARTP, as a novel mutagenesis tool, has a good application prospect.
This study aims to screen highly effective P-solubilizing strains of A. niger by ARTP mutagenesis and the peanut biomass and physiological indexes of the positive mutant strains were determined and investigated. This research provides a fundamental basis for the further development of multifunctional fungal agent and their applications. In addition, it provides a reference model and a method for the mutation breeding of other microorganisms.

Aspergillus niger strain and reagents
The original strain A. niger strain (xj) was isolated and identified by the Institute of Fungi Resource, Guizhou University, and stored at the China Center for Type Culture Collection (CCTCC NO. M206021) (Li et al., 2007). Chemical reagents of this experiment were purchased from Sinopharm Chemical Reagent Co., Ltd. (China).

Mutation of Aspergillus niger xj
The method of mutagenesis of strains referred to Zhang et al. (2019). Helium was used as the working gas and the mutagenic treatment distance was 2 mm, the processing power was 120 W, the gas flow rate was 10 slm (standard liter per minute), and the treatment time was from 0 s to 300 s with intervals of 30 s. The calculation of lethality rate was carried out following the protocol of Luo et al. (2018).
where U represents the number of unmutated colonies (0 s) and T represents the number of colonies after the mutagenesis.

Screening of positive mutant strains
Sterilized pikovskaya's agar medium was poured into sterilized petri dish. After solidification of the medium, a pinpoint inoculation of the single mutagenic colony of A. niger strain was made on the plates aseptically and incubated for 7 days at 28 C. The intensity of tricalcium phosphate solubilisation was measured as the diameter of the halozone formed around the colonies (Maurya & Kumar, 2006). The above method aims to primarily screened the mutagenesis strains with P-solubilization effect. The primary screening strains were selected with a better P dissolving ability for re-screening, and P content was determined by Mo-Sb Colorimetry (Li & Zheng, 2020). The genetic variability of the mutant strains induced by artificial mutagenesis was low and easy to repair or mutate. Therefore, the mutant strains were subcultured based on their genetic stability (Tao et al., 2004). In this study, the genetic stability of the mutant strain was evaluated by 10 passages. Values were shown as mean ± standard deviation (SD) from triplicately repeated experiments.

Measurement of organic acids
In this study, seven kinds of organic acids (oxalic acid, malic acid, citric acid, tartaric acid, lactic acid, acetic acid, and succinic acid) were determined by a method of Yang et al. (2018). The organic acid concentration as the independent variable x and the peak area as the dependent variable y, were taken to draw the standard curve by the external standard method. The unknown organic acids in culture filtrate were determined by comparing the retention times (RT) and peaks areas of chromatograms with the standard organic acids (Bakri, 2019).
Determination of indole-3-acetic acid (IAA) content IAA concentration (0,10,20,30,40, and 50 µg mL -1 ) was taken separately, and a volume of 4 mL Salkowski was added to the mixture to promote full reaction at 28 C for 30 min. IAA concentration was measured by UV-VIS Spectrophotometer (BIOMATE 3S; Thermo Fisher, Waltham, MA, USA) at 530 nm. IAA concentration as the abscissa x and the absorbance as the ordinate y to draw the IAA standard curve. A. niger spore suspension (10 8 CFU mL -1 ) was inoculated and incubated at 28 C and centrifuged at 150 r/min for 5 days. After that, it was centrifuged again at 109 g (Allegra X-30R; Beckman Coulter, Brea, CA, USA) for 10 min, mixed with liquid supernatant (1 mL) and Salkowski (4 mL) at 28 C for 30 min. Three technical replicates were done in the experiment, the IAA content was calculated by comparing the IAA standard curve.

Determination of phosphorus content
The determination of P content was carried out by the method of Zhang (2008). However, the absorbance of the sample was measured by UV spectrophotometer at 700 nm. The standard curve of phosphorus was drawn with P content as the abscissa x and absorption value as the ordinate y. The content of soluble P in the centrifugal supernatant was determined by Mo-Sb Colorimetry.

Determination of phosphorus removal kinetics curve of strains
The spore suspension was inoculated into a liquid medium containing 5% calcium phosphate. The culture solution was inoculated at 28 C and 150 r/min for 7 days. During the culturing, the samples were taken at regular intervals of 24 h to be centrifuged at 109 g for 5 min at 4 C. The concentration of spore suspension was set to 1 × 10 8 CFU/mL for xj90-32, xj120-12, xj120-31, and xj180-22 mutated strains. The content of soluble P in the centrifugal supernatant was determined and the value of pH was determined by pH meter (PHS-3C; Dapu Instrument, Shanghai, Co., Ltd., Shanghai, China).

Effect of different factors on the phosphorus-solubilizing ability of mutant strains
Studies have shown that the carbon source, nitrogen source, pH, and other factors of the culture medium would affect the P-solubilizing ability of P-solubilizing fungi (Patel, Archana & Kumar, 2008). Therefore, the mutagenic strains of A. niger need to investigate the influence of these factors on the ability of solubilizing P. These factors included (carbon source and concentration, nitrogen source and concentration, temperature, NaCl, initial pH). Effects of changes in carbon sources and concentration, nitrogen sources and concentration, temperature, salinity, initial pH on P-solubilizing abilities were evaluated using calcium phosphate medium. The type of carbon sources included glucose, sucrose, maltose, lactose, and starch, and concentration were 0.5%, 1%, 5%, 10% and 15%. Baseline experimental conditions were: concentration of A. niger spore suspension 1 × 10 8 CFU mL -1 , ammonium sulfate concentration 0.5 g L -1 , initial pH 7.5, NaCl 3 g L -1 , and incubated aerobically (150 rpm min -1 , 30 C) for 5 days. Nitrogen sources were derived from beef extract, sodium nitrate, ammonium sulfate, potassium nitrate, and carbamide, and concentration were 0%, 0.05%, 0.5%, 1%, 5% and 10%, NaCl concentrations were regulated to 0%, 0.5%, 1.5%, 2%, 3%, 4%, 5%, 6%, 8%, and 10%, initial pH was adjusted to 3, 5, 7, 9, and 11, and temperatures were changed to 20, 25, 30, 35, 40, and 50 C. The effects of all these factors on the P solubilization were separately determined. Other conditions are the same as for the above determination of P content. Values are shown by mean ± SD from triplicate experiments.

Collection of peanut samples and measurement of growth characteristics
Peanut seeds were firstly disinfected with hydrogen peroxide, rinsed with sterile water, and subjected to 28 C for 24 h to accelerate the germination. Subsequently, seeds were placed in a test pot containing 300 g of soil, which was collected from the campus of Guizhou University with the geographical coordinates of 106 66 E′ and 26 44 N′. The larger particles and debris were filtered, which were mixed with fine sand in a 1:2 (V:V) ratio. Besides, a certain amount of insoluble calcium phosphate was added to each pot of soil at the ratio of 1:1,000 (W:W). The A. niger positive mutant strains (10 6 CFU g -1 ) were inoculated with the peanut that was grown for 3 days, and the blank controls were prepared (inoculating the same amount of sterile water for CK control). When peanuts were growing up 30 days and was collected. Then, sterile water was used to clean the soil at the root of the peanut, and the filter paper was used to suck water. The growth indicators (plant height, root length, and dry and fresh biomass), chlorophyll content, and protein content were measured. the plant height and root length were measured by a ruler. Fresh biomass was measured with an analytical balance (BS110S; Sartorius Tianping, Co., Ltd., Beijing, China). Besides, the peanut was put into a sterilization carton and sterilized at 105 C for 20 min and dried at 80 C to constant weight. The dry biomass of the peanut was measured by analytical balance. Values shown are mean ± SD from triplicate experiments.

Determination of physiological indexes (chlorophyll and total protein content)
Around 100 g of peanut leaves were collected, washed, and dried. They were next cut into slices in 1-mm width and placed in a 10 mL test tube. Leaves were fully soaked in 2 mL of dimethyl sulfoxide (DMSO) at 65 C until they turned white or transparent. The extracted liquid was cooled to room temperature, and the extracted liquid was mixed fully with 80% acetone (8 mL) (Qiu et al., 2016). Chlorophyll concentration was determined using UV-VIS Spectrophotometer at 663.6 nm, and 646.6 nm and the calculation formula referred to Porra, Thompson & Kriedemann (1989).
The standard protein curve of bovine serum protein was made by a method of Bradford (1976). Around 0.5 g of fresh peanut leaves was taken, washed, and wipe-dried. The dried leaves were placed in a mortar and about 5 mL of phosphate buffer saline (PBS) was added to the mortar. Leaves were grounded to extract the protein, which was thoroughly mixed with Coomassie brilliant blue G-250 (0.1 mg mL -1 ) and stand for 5 min. The absorbance value was measured at 595 nm by UV-VIS Spectrophotometer and the protein content in the sample was calculated. The formula is as follows: The protein content of sample mg=g where C represents the protein content calculated by the standard protein curve, unit (µg); V T represents the total volume of the extract, unit (mL); V 1 represents the added sample amount when determination, unit (mL); FW represents the fresh weight of the sample, unit (g).
Effect of the Aspergillus niger spore suspension on available phosphorus content in the soil Soil samples were air-dried and filtered using a 1 mm sieve. Around 2 g of dried samples were transferred to a 100 mL conical flask filled with 20 mL of 0.50 mol L -1 sodium bicarbonate solution. Then, samples were put at 28 C and 150 r/min for 30 min. After, the samples were filtered and centrifuged at 109 g for 5 min. One mL of supernatant was used to determine the available P content by Mo-Sb Colorimetry. The test was performed in triplicate.

Statistical analysis
One-way analysis of variance (ANOVA) was performed for data analysis using IBM SPSS (ver. 23.0; SPSS Inc., Armonk, NY, USA). The differences among the groups were evaluated by Duncan's test, and p-value < 0.05 was considered significant.

Investigation of the ARTP mutagenesis time
The lethality rate of the strain increased with time. The positive mutation rate showed a trend of increase first and then a decrease. When the treatment time reached 120 s, the lethality rate was 37%, and the positive mutation rate was 25.5%. The treatment time was 240 s, the lethality rate was 85%, whereas the positive mutation rate was only 6.38%. Therefore, the treatment time with the highest positive mutation rate was considered as the best condition for the mutagenesis of the xj strain, and the treatment time was 120 s (Fig. 1).

Screening of mutagenic strains
Certain strains among a total of 670 mutant xj strains obtained by ARTP mutagenesis were efficient in solubilizing the inorganic phosphorus (calcium phosphate) in the medium. The 141 and 24 mutant strains were acquired by preliminary and secondary screening, respectively. The standard curve of P content was prepared and analyzed by linear regression, resulting in the following correlation model: y = 0.0103x + 0.0069, r = 0.994, which showed a good linear relationship and met the sample testing requirements. The analysis results revealed that the xj90-32, xj120-12, xj120-31, and xj180-22 strains did not show differences in P-solubilizing abilities within 10 generations, indicating that the four strains were good genetic stabilities and the P-solubilizing abilities increased by 50.3%, 57.5%, 55.9%, and 61.4%, respectively (Table 1).

Determination of organic acid contents
HPLC was used to analyze the organic acids in the medium containing calcium phosphate and revealed the P-solubilization mechanism of the xj strain. In this experiment, the standard curves of seven organic acids were prepared and analyzed by linear regression, resulting in the following coefficients: oxalic acid (y = 0.0987x + 0.2843, r = 0.9944), malic acid (y = 0.0228x + 0.118, r = 0.9995), citric acid (y = 0.0101x + 0.2628, r = 0.9984), tartaric acid (y = 0.0146x + 0.7278, r = 0.9946), lactic acid (y = 0.0057x + 0.2372, r = 0.9987), acetic acid (y = 0.0055x + 0.6848, r = 0.9951) and succinic acid (y = 0.0055x + 0.4042, r = 0.9983). All above-mentioned curves revealed close linear relationships, which met the requirements of samples testing. We observed differences in the kinds and contents of organic acids between the xj strain and the four positive mutant strains (Table 2).

Determination of IAA content
The standard curve of IAA was prepared and analyzed by linear correlation, resulting in the following coefficient: y = 0.0138x + 0.0138, and r = 0.9972. The curve displayed a good linear relationship, which met the requirements of sample testing. As shown in   tryptophan. The positive mutant strain xj120-12 exhibited a significant difference from xj strains (P < 0.05). The highest IAA content was 10.5%, which was higher than that in xj strain. However, strains of xj90-32, xj120-31, and xj180-22 were not significantly different from xj strains (P > 0.05).

Determination of kinetic curve of phosphorus solution
According to Fig. 3A, all strains started releasing soluble P into the culture medium on day first. On the fifth day, the soluble P content of xj, xj90-32, xj120-12, xj120-31, and xj180-22 strains reached the maximum values of 554.3 µg mL -1 , 744.4 µg mL -1 , 787.6 µg mL -1 , 769.9 µg mL -1 , and 810.9 µg mL -1 , respectively. Afterward, the P content began decreasing at 6 and 7 days affecting by time. Simultaneously, the pH value of five strains sharply decreased during the first 2 days and remained at a lower pH value from 2 to 7 days (Fig. 3B). During the dissolution of calcium phosphate, the soluble P content of five strains presented a relatively negative relationship with pH.

Effect of carbon sources on the phosphorus-solubilization ability of strain
The effects of different carbon sources (monosaccharides, disaccharides, and polysaccharides) on the ability of A. niger to dissolve calcium P were investigated. Effects of different carbon sources on the P content were significantly different in order, as follows: glucose > sucrose > maltose > starch > lactose (Fig. 4A). When glucose was used as the sole carbohydrate component, P content was the highest (P < 0.05). Compared with the xj strain, the P-solubilizing rates of four positive mutant strains marked as xj90-32, xj120-12, xj120-31, xj180-22 increased by 41.2%, 49.2%, 45.8%, and 52.4%, respectively. In addition, glucose concentration had a significant effect on the P-solubilizing ability of the strains. In the range of 5∼15%, the P-solubilizing increased with the increase of

Effect of nitrogen sources on the phosphorus-solubilization ability of strain
Nitrogen sources had different influences on the P removal ability of the strains. When ammonium sulfate was used as the nitrogen component, the P content was the highest (P < 0.05). In contrast to the xj strain, the xj90-32, xj120-12, xj120-31, and xj180-22 strains had higher P-solubilizing rates boosted by 40.5%, 49.1%, 46.6%, and 53.1%, respectively (Fig. 5A). Besides, when ammonium sulfate concentration was 0.5%, the P-solubilizing quantities of the mutant strains enhanced 34.1%, 41%, 36.6%, and 62.2%, respectively (Fig. 5B). Effect of NaCl, temperature and pH on the phosphorus-solubilization ability of strain The effects of different NaCl concentrations on the ability of strains to dissolve calcium P were determined. The P-solubilizing abilities of strains were the highest at lower NaCl concentration 1% (Fig. 6A). Compared to xj strain, the P-solubilizing quantities of strains (xj90-32, xj120-12, xj120-31, and xj180-22) increased by 40%, 47.1%, 43.4%, and 49.2%, respectively. The effect of temperature ranging from 20 to 50 C on the ability of A. niger to hydrolyze calcium phosphate was determined. The P-solubilizing ability was the highest at the temperature 35 C. Compared to the xj strain, P-solubilization quantities of strains (xj90-32, xj120-12, xj120-31, and xj180-22) increased by 27.4%, 36.9%, 30.2%, and 32.2%, respectively (Fig. 6B). To assess the pH adaptability of A. niger strains during P solubilization, the effect of pH (ranging from 3 to 11) on the ability of five strains to dissolve calcium P was determined. The P-solubilizing abilities of strains had the highest at pH 7.0. Compared to the xj strain, the P-solubilization quantities of strains (xj90-32, xj120-12, xj120-31, and xj180-22) enhanced 40%, 44.3%, 43.5%, and 50%, respectively (Fig. 6C).

Effect of mutant positive strain on physiological indexes
The strains influenced the physiological indexes of peanuts, including chlorophyll and soluble protein content (Fig 8). The xj180-22 and xj120-12 strains improved the chlorophyll content compared with the CK (P < 0.05) by 49.5% and 27.9%, respectively. The enhancements were 36% and 16%, respectively, higher than the xj strain (Fig. 8A). In addition, the positive mutant strains increased soluble protein content than the CK (P < 0.05). The soluble protein content of xj180-22, xj120-31, xj120-12, and xj90-32 strains increased 12%, 10.7%, 9.2%, and 6%, respectively, than the CK. However, compared with the xj strain, the soluble protein contents were not significantly different in all the positive mutant strains (P > 0.05) (Fig. 8B).

Effect of mutant strain on the available phosphorus content in the soil
The available P content in soil for the CK was 6.88 mg kg -1 , which was considered low. The inoculation with the xj spore suspension increased the P content to 12.85 mg kg -1 . The xj120-12, xj120-31, xj90-32 and xj180-22 increased by 169.4%, 127.6%, 121.3% and 98.3%, respectively, higher than CK (P < 0.05). In addition, the xj120-12, xj120-31 and xj90-32 boosted 44.3%, 21.9%, and 18.5%, respectively higher than the xj strain (P < 0.05) (Fig. 9). In general, inoculation with the mutant strains xj120-12 could improve the P content in soils and promote peanut growth.

DISCUSSION
With the establishment of ARTP mutation and using primary screening, re-screening and subcultured 10 passages, we eventually obtained four representative mutants: xj90-32, xj120-12, xj120-31, and xj180-22. The positive mutation rate was 25.5%, when the optimal treatment time was 120 s. The good genetically stable of four strains were obtained, and the P-solubilization abilities increased more than 50%. Due to the occurrence of positive mutations is related to the mutagenic parameters and characteristics of the strain (Zhang et al., 2019). The positive mutation rate of strains were the highest in the study when the fatality rate was 37%.
With the decrease in the pH value, P content increased by contrast. This indicated that pH could be related to the P-solubilization ability of the mutant strain. Several reports have revealed that pH decreased due to the release of organic acids (Nath, Sharma & Barooah, 2012;Padamavathi, 2015;Whitelaw, 2000). Oxalic acid and critic acid were detected in four positive mutant strains and the xj strain. In addition, succinic acids were also secreted by xj120-12. The nature of organic acid produced is a specific characteristic of each fungal isolate but may vary under different cultivation conditions. Arguably, the mutagenesis treatment affected the kinds of organic acid, resulting in differences in metabolic capabilities and affecting the P-solubilization ability of mutant strains.
P-solubilization is a complex phenomenon that depends on many factors such as the culture's nutritional, physiological, and growth conditions (Isbelia et al., 1999). In this experiment, the kinetics curve showed an optimal culture time of 5 days, which was taken as the optimal culture time for the influencing factors. Glucose was used as a carbon source, and the P-solubilization abilities were obviously increased. Glucose is a monosaccharide with a simple structure and facilitates the acid production for the strain . Using ammonium sulfate as nitrogen sources also caused high P-solubilization efficiency. Similar results have been reported in previous studies that nitrogen in the ammonium form is necessary for P solubilization in organic acid production through NH + 4 /H + exchange mechanisms (Omar, 1997). The P-solubilizing abilities of the four mutant strains were the highest at 1% NaCl concentration, afterward, decreased with the NaCl concentration increase. These results were similar to the of Srividya, Soumya & Pooja (2009). The reason is that too much chloride ions may chelate or neutralize proton ions or acid produced in the media then, decrease the P-solubilizing ability. Except for carbon source, nitrogen source type and concentration and NaCl concentration, the formation process, and growth of A. niger mycelium will be affected by temperature and pH value. In this study, the P-solubilizing ability started decreasing with temperature and pH value over 35 C and 7, suggesting that microbial metabolism and biological activity affected the P-solubilizing ability of the strain. In summary, choosing the composition of the medium and conditions would increase the strains' P-solubilization ability; thus, improving the utilization rate of P in the soil (Liu et al., 2015).
The four positive mutant strains could increase in different degrees on height, root length, and dry and fresh biomass of peanut. The reason may be that the strains secreted IAA. According to reports, IAA is an endogenous plant growth hormone, promoting seed germination and thus plant growth (Wu et al., 2014). The xj180-22 and xj120-12 strains could improve the chlorophyll content. The cause is that chlorophyll is the most important pigment in plant photosynthesis, and its content is positively correlated with leaf color, which can roughly reflect the nutritional status of plants and affect the photosynthetic rate of plants (Zhang, Zhang & Li, 2008). The soluble protein as a kind of nutrient substance could directly affect the respiration of plants and catalyze all kinds of chemical reactions (Berry, 1982). In this study, the four mutant strains improved the soluble protein content compared with the CK. Besides, the xj120-12 strain improved the P content in the soil.

CONCLUSIONS
To sum up, the xj120-12 can be used as the dominant fungi with the potential of P solubilization and growth promotion and provided the basis for the production of P solubilization fungal fertilizer.

Competing Interests
We have a patent number for the Aspergillus niger xj strain (CN1847388).

Author Contributions
Qiuju Peng conceived and designed the experiments, performed the experiments, analyzed the data, prepared figures and/or tables, authored or reviewed drafts of the paper, and approved the final draft. Yang Xiao conceived and designed the experiments, performed the experiments, analyzed the data, prepared figures and/or tables, authored or reviewed drafts of the paper, and approved the final draft. Su Zhang conceived and designed the experiments, performed the experiments, prepared figures and/or tables, and approved the final draft.
Changwei Zhou conceived and designed the experiments, prepared figures and/or tables, and approved the final draft. Ailin Xie conceived and designed the experiments, authored or reviewed drafts of the paper, and approved the final draft. Zhu Li analyzed the data, authored or reviewed drafts of the paper, and approved the final draft. Aijuan Tan analyzed the data, authored or reviewed drafts of the paper, and approved the final draft. Lihong Zhou analyzed the data, prepared figures and/or tables, and approved the final draft. Yudan Xie analyzed the data, prepared figures and/or tables, and approved the final draft. Jinyi Zhao analyzed the data, prepared figures and/or tables, and approved the final draft. Chenglin Wu performed the experiments, authored or reviewed drafts of the paper, and approved the final draft. Lei Luo analyzed the data, prepared figures and/or tables, and approved the final draft. Jie Huang analyzed the data, prepared figures and/or tables, and approved the final draft. Tengxia He performed the experiments, authored or reviewed drafts of the paper, and approved the final draft. Ran Sun performed the experiments, authored or reviewed drafts of the paper, and approved the final draft.

Patent Disclosures
The following patent dependencies were disclosed by the authors: Aspergillus niger xj strain patent number: CN1847388.