利用本地分离真菌进行固态发酵并优化纤维素酶的生产

IF 0.7 Q4 PHARMACOLOGY & PHARMACY Egyptian Pharmaceutical Journal Pub Date : 2023-07-01 DOI:10.4103/epj.epj_30_23
Maha Basha, Y. Shetaia, Fathy Mehaya, Fatma Abdelzaher
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Cellulase production by tested fungal isolates was carried out through utilization of olive (Olea europaea), black seeds (Nigella sativa), and castor bean (Ricinus communis) cakes in SSF. Optimization of the cellulase productivity was performed by Plackett–Burman design (PBD) and Box–Behnken design. Results and conclusion Out of the isolated 35 fungi, only 12 (34%) produced cellulase in SSF using olive, black seeds (Nigella), and castor bean cakes. Out of these fungal isolates, only 4, that is, no. 1, 7, 10, and 17 were superior in reducing sugar production from olive cakes (13.04, 15.61, 17.03, and 12.85 mg/ml), respectively. While four fungal isolates no. (1, 7, 7, and 10) were active producers of reducing sugars from black seeds (15.45, 18.96, 20, and 18.08 mg/ml), respectively. Only a fungal isolate no. 7 gave high reducing sugars (15.34 mg/ml) in castor cake SSF. 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引用次数: 0

摘要

背景 纤维素酶是许多纤维素废物生物转化过程中使用最多的工业酶。本研究利用药用植物固体废弃物,研究了真菌在固态发酵(SSF)中生产纤维素酶的经济性。本研究的主要目标是优化生产纤维素酶的生长条件。目的 本研究旨在分离和筛选有能力生产降解药用植物固体废弃物酶的真菌分离物,并优化影响纤维素酶生产的生长因子。材料和方法 从不同来源通过平板法分离出 35 种真菌,并使用添加了 1%纤维素的 Czapek-Dox 肉汤培养基对其纤维素酶活性进行筛选。通过在 SSF 中利用橄榄(Olea europaea)、黑籽(Nigella sativa)和蓖麻(Ricinus communis)饼,测试了真菌分离物生产纤维素酶的情况。通过普拉克特-伯曼设计(PBD)和方框-贝肯设计对纤维素酶生产率进行了优化。结果与结论 在分离出的 35 种真菌中,只有 12 种(34%)在使用橄榄、黑籽(Nigella)和蓖麻饼的 SSF 中产生了纤维素酶。在这些真菌分离物中,只有 4 个真菌分离物,即 1 号、7 号、10 号和 17 号,在从橄榄饼中产生还原糖方面具有优势(分别为 13.04、15.61、17.03 和 12.85 毫克/毫升)。而四种真菌分离物(1、7、7 和 10)则是黑籽还原糖的积极生产者(分别为 15.45、18.96、20 和 18.08 毫克/毫升)。只有一种真菌分离物 No.只有 7 号真菌分离物在蓖麻饼 SSF 中产生了较高的还原糖(15.34 毫克/毫升)。最有效的真菌分离物(10 号)使用黑籽饼作为 SSF 的底物,产生了 20 毫克/毫升的还原糖。根据提取的真菌 DNA,使用特异的内部转录间隔引物(ITS1/ITS4)进行 PCR 扩增,鉴定出潜在的真菌分离物为赤曲霉(OQ085169)。对 PCR 产物进行了测序,并与 GenBank(NCBI)中的其他相关序列进行了比较。利用 PBD 对七个因素进行筛选后发现,只有三个变量:pH 值、培养时间和通气速率(rpm)对纤维素酶的产量有显著影响。根据 PBD 的结果,采用盒-贝肯设计来估计所选变量的最佳水平。使用 A. terreus (OQ085169),所有变量都明显增加了纤维素酶的产量。P 值非常低(0.0207),表明预测值和实际值之间存在显著的高度相关性(R2=0.98),这表明纤维素酶活性的 98% 的变化是由所选的自变量造成的。
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Solid-state fermentation and optimization of cellulase production using local fungal isolate
Background Cellulase is the most employed industrial enzyme in biological conversion of many cellulosic wastes. In this work, economic cellulase production by fungi in solid-state fermentation (SSF) by using solid wastes of medicinal plants was studied. Optimization of growth conditions for production of cellulase was the main target of this study. Objective The current study aimed to isolate and screen fungal isolates that have the ability to produce enzymes to degrade solid wastes of medicinal plant process and optimization of growth factors that affect cellulase production. Materials and methods Thirty-five fungal isolates were isolated from different sources by plating and screened for their cellulase activities using Czapek–Dox broth medium amended with 1% cellulose. Cellulase production by tested fungal isolates was carried out through utilization of olive (Olea europaea), black seeds (Nigella sativa), and castor bean (Ricinus communis) cakes in SSF. Optimization of the cellulase productivity was performed by Plackett–Burman design (PBD) and Box–Behnken design. Results and conclusion Out of the isolated 35 fungi, only 12 (34%) produced cellulase in SSF using olive, black seeds (Nigella), and castor bean cakes. Out of these fungal isolates, only 4, that is, no. 1, 7, 10, and 17 were superior in reducing sugar production from olive cakes (13.04, 15.61, 17.03, and 12.85 mg/ml), respectively. While four fungal isolates no. (1, 7, 7, and 10) were active producers of reducing sugars from black seeds (15.45, 18.96, 20, and 18.08 mg/ml), respectively. Only a fungal isolate no. 7 gave high reducing sugars (15.34 mg/ml) in castor cake SSF. The most potent fungal isolate (no. 10) produced 20 mg/ml of reducing sugars using black seed cakes as substrate for SSF. The potential fungal isolate was identified as Aspergillus terreus (OQ085169) based on the extracted fungal DNA that was amplified by PCR using specific internal-transcribed spacer primer (ITS1/ITS4). The PCR products were sequenced and compared with the other related sequences in GenBank (NCBI). The screening of seven factors using PBD showed that only three variables: pH, incubation time, and aeration rate (rpm) affected significantly cellulase production. Box–Behnken design was used to estimate the optimal level of the selected variables based on the results of the PBD. All variables increased significantly cellulase using A. terreus (OQ085169). The P value was very low (0.0207) that indicated the significant, high correlation between the predicted and actual values (R2=0.98), this indicating 98% of the variation in the cellulase activity was owing to the selected independent variables.
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来源期刊
Egyptian Pharmaceutical Journal
Egyptian Pharmaceutical Journal PHARMACOLOGY & PHARMACY-
CiteScore
1.10
自引率
0.00%
发文量
37
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