Suspension culture of stem cells established of Calendula officinalis L.

Plant gene editing is usually carried out by delivering reagents such as Cas9 and sgRNAs to explants in culture. Edited cells are then induced to differentiate into whole plants by exposure to various hormones. Creating edited plants through tissue culture is often inefficient, requires considerable time, only works with limited species and genotypes and causes unintended changes to the genome and epigenome. We report methods to generate gene edited dicotyledonous plants through de novo meristem induction. Developmental regulators and gene editing reagents are delivered to somatic cells on whole plants. Meristems are induced that produce shoots with targeted DNA modifications, and gene edits are transmitted to the next generation. The de novo induction of gene edited meristems sidesteps the need for tissue culture, promising to overcome a bottleneck in plant gene-editing.

Cell cycling plays an important role in plant development, including: (1) organ morphogenesis, (2) cell proliferation within tissues, and (3) cell differentiation. In this study we use a cyclin::beta-glucuronidase reporter construct to characterize spatial and temporal patterns of cell cycling at each of these levels during wild-type development in the model genetic organism Arabidopsis thaliana (Columbia). We show that a key morphogenetic event in leaf development, blade formation, is highly correlated with localized cell cycling at the primordium margin. However, tissue layers are established by a more diffuse distribution of cycling cells that does not directly involve the marginal zone. During leaf expansion, tissue proliferation shows a strong longitudinal gradient, with basiplastic polarity. Tissue layers differ in pattern of proliferative cell divisions: cell cycling of palisade mesophyll precursors is prolonged in comparison to that of pavement cells of the adjacent epidermal layers, and cells exit the cycle at different characteristic sizes. Cell divisions directly related to formation of stomates and of vascular tissue from their respective precursors occur throughout the period of leaf extension, so that differing tissue patterns reflect superposition of cycling related to cell differentiation on more general tissue proliferation. Our results indicate that cell cycling related to leaf morphogenesis, tissue-specific patterns of cell proliferation, and cell differentiation occurs concurrently during leaf development and suggest that unique regulatory pathways may operate at each level. Copyright 1999 Academic Press.