Development of a set of novel binary expression vectors for plant gene function analysis and genetic transformation

Xiuyuan Wang; Chong Teng; Huitian Wei; Shuang Liu; Hongzhuan Xuan; Wentao Peng; Qianqian Li; Hongyan Hao; Qingya Lyu; Shanhua Lyu; Yinglun Fan

doi:10.3389/fpls.2022.1104905

Development of a set of novel binary expression vectors for plant gene function analysis and genetic transformation

Front Plant Sci. 2023 Jan 12:13:1104905. doi: 10.3389/fpls.2022.1104905. eCollection 2022.

Authors

Affiliation

¹ College of Agriculture, Liaocheng University, Liaocheng, China.

Abstract

With the advent of multiple omics and Genome-Wide Association Studies (GWAS) technology, genome-scale functional analysis of candidate genes is to be conducted in diverse plant species. Construction of plant binary expression vectors is the prerequisite for gene function analysis. Therefore, it is of significance to develop a set of plant binary expression vectors with highly efficient, inexpensive, and convenient cloning method, and easy-to-use in screening of positive recombinant in Escherichia coli. In this study, we developed a set of plant binary expression vectors, termed pBTR vectors, based on Golden Gate cloning using BsaI restriction site. Foreign DNA fragment of interest (FDI) can be cloned into the destination pBTR by one-step digestion-ligation reaction in a single tube, and even the FDI contains internal BsaI site(s). Markedly, in one digestion-ligation reaction, multiple FDIs (exemplified by cloning four soybean Glyma.02g025400, Glyma.05g201700, Glyma.06g165700, and Glyma.17g095000 genes) can be cloned into the pBTR vector to generate multiple corresponding expression constructs (each expression vector carrying an FDI). In addition, the pBTR vectors carry the visual marker, a brightness monomeric red fluorescent protein mScarlet-I, that can be observed with the unaided eye in screening of positive recombinants without the use of additional reagents/equipment. The reliability of the pBTR vectors was validated in plants by overexpression of AtMyb75/PAP1 in tomato and GUSPlus in soybean roots via Agrobacterium rhizogenes-mediated transformation, promoter activity analysis of AtGCSpro in Arabidopsis via A. tumefaciens-mediated transformation, and protein subcellular localization of the Vitis vinifera VvCEB1_opt in tobacco, respectively. These results demonstrated that the pBTR vectors can be used in analysis of gene (over)expression, promoter activity, and protein subcellular localization. These vectors will contribute to speeding up gene function analysis and the process of plant molecular breeding.

Keywords: golden gate cloning; mScarlet-I gene; one-step digestion-ligation reaction; plant binary expression vector; visible selection marker.

Grants and funding

This work was supported by National Natural Science Foundation of China (No. 31271751); Partial financial support was received from Industrial upgrading project of Shandong Agricultural Science and Technology (2019YQ035); and Innovation Project for an undergraduate to QYL (no. CYCY2022412).