Glossary on genome editing

A variant form of a gene at a particular locus on a chromosome. Different alleles produce variations in inherited characteristics.

Base editing is a genome editing method based on CRISPR/Cas9. It allows the targeted and directed conversion of one DNA or RNA base into another (i.e. the introduction of a point mutation) using DNA or RNA base editors. These base editors comprise a catalytically disabled nuclease fused to a catalytically active nucleobase deaminase enzyme.

A thread-like structure that contains a single length of DNA, usually carrying many hundreds of genes. Different plants have different number of chromosomes: for example, sugarbeet has 18 chromosomes. Plants also vary in terms of ploidy, i.e., the number of sets of chromosomes.

Chromosomes usually reside in the nucleus of a cell. Besides chromosomes, also the plants’ organelles (mitochondria and chloroplasts) contain DNA.

An adaptive component of bacterial and archaeal immune systems, used as a method of genome editing. CRISPR (Clustered Regularly Interspaced Short Palindromic Repeats) describes a segment of repetitive sequences separated by (foreign) viral DNA (called spacer). Proteins associated with CRISPR (Cas) use these specific sequences to protect the cell by finding and destroying viral DNA.

The organism from which genetic material is obtained for transfer to the recipient organism.

A change to the DNA sequence (e.g. insertion, deletion, substitution) at a specific site in the genome that is produced with targeted mutagenesis methods of genome editing and results in an intended effect (e.g. gene disruption).

A protein acting as a biological catalyst for chemical reactions.

A functional unit of heredity that is a segment of DNA in a specific part of a chromosome. A gene typically directs the formation of a protein or RNA molecule.

Germplasm (i.e. genetic material) within which sexual recombination is possible as a result of hybridization, including via methods such as embryo culture.

Biological organism whose genetic material has been changed in such a way, which would not be possible under natural conditions like crossing or natural recombination.

The complete DNA of an organism. Plant genomes are highly variable in size.

The term includes several new methods, with which targeted and site-specific double-strand breaks are induced in the DNA. Due to the cell`s own but often error-prone DNA repair mechanism (NHEJ: non-homologous end-joining), double-strand breaks may result in mutations (InDels, SNPs). In the presence of a repair template, the (cellular) precise mechanism of homologous recombination (HR) can be used to implement specific changes in the DNA or to insert entire genes. The methods grouped under this term are CRISPR/Cas, TALENs, ZFNs, meganucleases and ODM.

The genetic constitution of an organism.

Short segments of RNA used to direct the DNA cutting protein to the target location in the genome. gRNA segments contain the region of homology to the target sequence (usually 20 bases), and a sequence that interacts with the nuclease (e.g. Cas9).

Having different variants (alleles) of a specific gene on the homologous chromosomes of a cell or an organism.

Repair mechanism of the cell for DNA strand breaks which uses a segment of homologous donor DNA (acting as a repair template), “patching” the DNA. The repair template donor DNA must have major similarities to the cleavage sites of the DNA in its sequences (homologies) to be able to be inserted. HR is a more precise repair than NHEJ. During genome editing, the donor DNA is designed and inserted in a targeted manner; hence, it could potentially replace a pathological gene with a healthy copy.

Having the same variant (allele) of a specific gene on homologous chromosomes of a cell or an organism.

A line that has been selfed to sufficient homozygosity to be considered homozygote.

Abbreviation for insertion and/or deletion. Describes the random removal or introduction of nucleotides in the DNA sequence. InDels occur when DNA double-strands are inaccurately repaired by NHEJ. This often leads to the disruption of the open reading frame and/or the creation of premature stop codons and therefore a loss of gene function.

Any new combination of genes and regulatory elements of that same species that were combined outside the organism and incorporated into the plant genome where they are capable of continued propagation.

A type of enzyme that binds to and cuts DNA at specific DNA sequences. Meganucleases can be used in genome editing for both nonhomologous end joining (NHEJ) and homology directed repair-mediated alterations.

A change of an organism´s own DNA sequence. The change can be small (SNPs, small InDels) or can span thousands of base pairs (insertions, deletions, translocations, replacements) or can affect whole chromosomes but is limited to sequence variations within the gene pool (crossable species).

An enzyme that can cut through DNA or RNA strands.

A direct or indirect, unintended, short- or long-term consequence of an intervention on an organism other than the intended effect on that organism. For example, when a genome editing enzyme cuts DNA at an unintended, "off-target," site that is similar to the intended target.

Different observable characteristics that can be produced by two or more alleles of a genetic locus within a species that control a trait which is the result of the underlying genotype and its interaction with the environment. For example, flower colour is a trait, and red and white flower colours are two different phenotypes for the flower colour trait.

In nature, a plasmid is a small DNA molecule within a cell that is physically separated from chromosomal DNA and can replicate independently from genomic DNA. Plasmids are most commonly found as small circular, double-stranded DNA molecules in bacteria. In genetic engineering, isolated, artificial plasmids are widely used as vectors in molecular cloning.

Prime editing is a CRISPR/Cas9-based system that rewrites DNA to induce targeted and precise insertions, deletions, and base-to-base conversions. This method uses a prime editing guide RNA (pegRNA), a catalytically impaired Cas9 nuclease, and an engineered reverse transcriptase that initiates the precise change, addition or removal of a sequences. Once the new genetic material is incorporated into the cut strand of DNA, the prime editor nicks the unedited strand, signalling to the cell to rebuild it to match the edited strand.

Produced by joining two or more nucleic acid molecules by whatever means outside an organism capable of continued propagation after incorporation into an organism (in accordance to BVL, 2017).

A nucleic acid sequence used to direct cellular DNA repair pathways to incorporate specific DNA sequence changes at or near a target site.

A single-stranded molecule that transmits and regulates the DNA’s instructions for the development, functioning, and reproduction of all living organisms.

RNAi is a naturally occurring mechanism for gene silencing, triggered by double-stranded RNA (dsRNA). RNAi processes can be used by researchers to block, or silence, the expression of a given gene.

Methods which induce double-strand breaks at specific and defined points of the genome by means of endonucleases. The DNA-binding domain can be either a protein or RNA. Methods that fall under this umbrella term are CRISPR/Cas, TALENs and ZFNs. SDN is subdivided into SDN-1, SDN-2 and SDN-3, depending on the degree of induced change.

The process of generating a mutation at a predefined location within a genome by using genome editing methods. The resulting mutation can be random (by using SDN-1) or specific (by using e.g., Base Editing, SDN-2 or SDN-3). Sequence insertions and replacements through targeted mutagenesis are limited to sequence variations within the gene pool (crossable species). The obtained changes could have been the result of traditional breeding or of a natural mutation.

A nucleic acid sequence subject to intentional binding, modification, or cleavage.

An observable (able to be seen or otherwise identified) characteristic of an organism. For example, flower colour is a trait.

An organism into which one or more genes have been transferred or introduced from another species of organism (GMO).

A distinct, uniform, stable genotype approved for its value for cultivation and use.