A CRISPR/Cas9-based visual toolkit enabling multiplex integration at specific genomic loci in Aspergillus niger

IF 4.4 2区生物学 Q1 BIOTECHNOLOGY & APPLIED MICROBIOLOGY

Synthetic and Systems Biotechnology Pub Date : 2024-02-10 DOI:10.1016/j.synbio.2024.01.014

Yangyang Li , Cen Li , Yishan Fu , Quan Zhang , Jianing Ma , Jingwen Zhou , Jianghua Li , Guocheng Du , Song Liu

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Abstract

Aspergillus niger is a highly versatile fungal strain utilized in industrial production. The expression levels of recombinant genes in A. niger can be enhanced by increasing the copy number. Nevertheless, given the prolonged gene editing cycle of A. niger, a “one-step” strategy facilitating the simultaneous integration of recombinant genes into multiple genomic loci would provide a definitive advantage. In our previous study, a visual multigene editing system (VMS) was designed to knock out five genes, employing a tRNA-sgRNA array that includes the pigment gene albA and the target genes. Building upon this system, hybrid donor DNAs (dDNAs) were introduced to establish a clustered regularly interspaced short palindromic repeats (CRISPR)-based multiplex integration toolkit. Firstly, a CRISPR-Cas9 homology-directed repair (CRISPR-HDR) system was constructed in A. niger by co-transforming the CRISPR-Cas9 plasmid (with a highly efficient sgRNA) and the dDNA, resulting in precise integration of recombinant xylanase gene xynA into the target loci (the β-glucosidase gene bgl, the amylase gene amyA, and the acid amylase gene ammA). Subsequently, the length of homology arms in the dDNA was optimized to achieve 100% editing efficiency at each of the three gene loci. To achieve efficient multiplex integration in A. niger, the CRISPR plasmid pLM2 carrying a sgRNA-tRNA array was employed for concurrent double-strand breaks at multiple loci (bgl, amyA, ammA, and albA). Hybrid dDNAs were then employed for repair, including dDNA1-3 (containing xynA expression cassettes without selection markers) and dDNA_albA (for albA knockout). Among the obtained white colonies (RLM2′), 23.5% exhibited concurrent replacement of the bgl, amyA, and ammA genes with xynA (three copies). Notably, the xynA activity obtained by simultaneous insertion into three loci was 48.6% higher compared to that obtained by insertion into only the bgl locus. Furthermore, this multiple integration toolkit successfully enhanced the expression of endogenous pectinase pelA and Candida antarctica lipase CALB. Hence, the combined application of VMS and the CRISPR-HDR system enabled the simultaneous application of multiple selection markers, facilitating the rapid generation in the A. niger cell factories.

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基于 CRISPR/Cas9 的可视化工具包，实现黑曲霉特定基因组位点的多重整合

黑曲霉是一种用途广泛的真菌菌株，可用于工业生产。黑曲霉中重组基因的表达水平可以通过增加拷贝数来提高。然而，鉴于黑曲霉的基因编辑周期较长，一种能将重组基因同时整合到多个基因组位点的 "一步到位 "策略将带来明显的优势。在我们之前的研究中，我们设计了一种可视化多基因编辑系统（VMS），利用包括色素基因 albA 和目标基因在内的 tRNA-sgRNA 阵列来敲除五个基因。在这一系统的基础上，引入了杂交供体DNA（dDNA），以建立基于聚类规则间隔短回文重复序列（CRISPR）的多重整合工具包。首先，通过CRISPR-Cas9质粒（含有高效sgRNA）和dDNA的共转化，在黑曲霉中构建了CRISPR-Cas9同源定向修复（CRISPR-HDR）系统，从而将重组木聚糖酶基因xynA精确整合到目标基因座（β-葡萄糖苷酶基因bgl、淀粉酶基因amyA和酸性淀粉酶基因ammA）。随后，对 dDNA 中同源臂的长度进行了优化，使三个基因位点的编辑效率均达到 100%。为了在黑僵菌中实现高效的多重整合，采用了携带 sgRNA-tRNA 阵列的 CRISPR 质粒 pLM2，在多个基因位点（bgl、amyA、ammA 和 albA）同时进行双链断裂。然后采用混合 dDNA 进行修复，包括 dDNA1-3（含有 xynA 表达盒，不含选择标记）和 dDNAalbA（用于 albA 基因敲除）。在获得的白色菌落（RLM2′）中，23.5%的菌落同时用 xynA（三个拷贝）替换了 bgl、amyA 和 ammA 基因。值得注意的是，与只插入 bgl 基因座相比，同时插入三个基因座获得的 xynA 活性高出 48.6%。此外，这种多重整合工具包还成功地提高了内源果胶酶 pelA 和白色念珠菌脂肪酶 CALB 的表达。因此，联合应用 VMS 和 CRISPR-HDR 系统可以同时应用多种选择标记，促进黑曲霉细胞工厂的快速生成。

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来源期刊

Synthetic and Systems Biotechnology BIOTECHNOLOGY & APPLIED MICROBIOLOGY-

CiteScore

6.90

自引率

12.50%

发文量

审稿时长

67 days

期刊介绍： Synthetic and Systems Biotechnology aims to promote the communication of original research in synthetic and systems biology, with strong emphasis on applications towards biotechnology. This journal is a quarterly peer-reviewed journal led by Editor-in-Chief Lixin Zhang. The journal publishes high-quality research; focusing on integrative approaches to enable the understanding and design of biological systems, and research to develop the application of systems and synthetic biology to natural systems. This journal will publish Articles, Short notes, Methods, Mini Reviews, Commentary and Conference reviews.