A novel microplate‐based screening strategy to assess the cellulolytic potential of Trichoderma strains

纤维素酶 木霉菌 生物转化 食品科学 化学 哈茨木霉 纤维素 色谱法 生物 微生物学 发酵 生物化学 生物技术 植物 生物病虫害防治
作者
Stefano Cianchetta,S. Galletti,P. L. Burzi,C. Cerato
出处
期刊:Biotechnology and Bioengineering [Wiley]
卷期号:107 (3): 461-468 被引量:36
标识
DOI:10.1002/bit.22816
摘要

Abstract Bioconversion of lignocellulosic biomass to fuel requires a hydrolysis step to obtain fermentable sugars, generally accomplished by fungal enzymes. An assorted library of cellulolytic microbial strains should facilitate the development of optimal enzyme cocktails specific for locally available feedstocks. Only a limited number of strains can be simultaneously assayed in screening based on large volume cultivation methods, as in shake flasks. This study describes a miniaturization strategy aimed at allowing parallel assessment of large numbers of fungal strains. Trichoderma strains were cultivated stationary on microcrystalline cellulose using flat bottom 24‐well plates containing an agarized medium. Supernatants obtained by a rapid centrifugation step of the whole culture plates were evaluated for extracellular total cellulase activity, measured as filter paper activity, using a microplate‐based assay. The results obtained were consistent with those observed in shake‐flask experiments and more than 300 Trichoderma strains were accordingly characterized for cellulase production. Five strains, displaying on shake‐flasks at least 80% of the activity shown by the hyper‐cellulolytic mutant Trichoderma Rut‐C30, were correctly recognized by the screening on 24‐well plates, demonstrating the feasibility of this approach. Cellulase activity distribution for the entire Trichoderma collection is also reported. One strain ( T. harzianum Ba8/86) displayed the closest profile to the reference strain Rut‐C30 in time course experiments. The method is scalable and addresses a major bottleneck in screening programs, allowing small‐scale parallel cultivation and rapid supernatant extraction. It can also be easily integrated with high‐throughput enzyme assays and could be suitable for automation. Biotechnol. Bioeng. 2010;107: 461–468. © 2010 Wiley Periodicals, Inc.
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