Institute of Biology Leiden, Department of Molecular Microbiology and Biotechnology, Sylvius Laboratory, Sylviusweg 72, Leiden, Netherlands.
Appl Environ Microbiol. 2010 Aug;76(16):5344-55. doi: 10.1128/AEM.00450-10. Epub 2010 Jun 18.
The physiology of filamentous fungi at growth rates approaching zero has been subject to limited study and exploitation. With the aim of uncoupling product formation from growth, we have revisited and improved the retentostat cultivation method for Aspergillus niger. A new retention device was designed allowing reliable and nearly complete cell retention even at high flow rates. Transcriptomic analysis was used to explore the potential for product formation at very low specific growth rates. The carbon- and energy-limited retentostat cultures were highly reproducible. While the specific growth rate approached zero (<0.005 h(-1)), the growth yield stabilized at a minimum (0.20 g of dry weight per g of maltose). The severe limitation led to asexual differentiation, and the supplied substrate was used for spore formation and secondary metabolism. Three physiologically distinct phases of the retentostat cultures were subjected to genome-wide transcriptomic analysis. The severe substrate limitation and sporulation were clearly reflected in the transcriptome. The transition from vegetative to reproductive growth was characterized by downregulation of genes encoding secreted substrate hydrolases and cell cycle genes and upregulation of many genes encoding secreted small cysteine-rich proteins and secondary metabolism genes. Transcription of known secretory pathway genes suggests that A. niger becomes adapted to secretion of small cysteine-rich proteins. The perspective is that A. niger cultures as they approach a zero growth rate can be used as a cell factory for production of secondary metabolites and cysteine-rich proteins. We propose that the improved retentostat method can be used in fundamental studies of differentiation and is applicable to filamentous fungi in general.
丝状真菌在接近零生长速率下的生理学特性一直受到有限的研究和利用。为了将产物形成与生长解耦,我们重新审视并改进了黑曲霉的恒化器培养方法。设计了一种新的保留装置,即使在高流速下也能可靠且几乎完全保留细胞。转录组分析用于探索极低比生长速率下产物形成的潜力。碳和能量有限的恒化器培养具有高度可重复性。虽然比生长速率接近零(<0.005 h(-1)),但生长产率稳定在最小值(每克麦芽糖产生 0.20 克干重)。严重的限制导致了无性分化,并且所供应的基质被用于孢子形成和次生代谢。恒化器培养的三个生理上不同的阶段都进行了全基因组转录组分析。严重的基质限制和孢子形成在转录组中得到了清晰的反映。从营养生长到生殖生长的转变的特征是编码分泌基质水解酶和细胞周期基因的下调,以及编码分泌小半胱氨酸丰富蛋白和次生代谢基因的许多基因的上调。已知分泌途径基因的转录表明,黑曲霉适应于小半胱氨酸丰富蛋白的分泌。从这个角度来看,接近零生长速率的黑曲霉培养可以用作生产次生代谢物和富含半胱氨酸的蛋白质的细胞工厂。我们提出,改进的恒化器方法可用于分化的基础研究,并且适用于一般的丝状真菌。