Table 2.
Tabular presentation of comparative attributes of plant genome editing techniques.
| CRISPR/Cas9 | Zinc Finger Nucleases (ZFNs) | Transcription factor like effector nucleases (TALENs) | Reference | |
|---|---|---|---|---|
| Mode of action | It works by inducing double-strand breaks in target DNA or single-strand DNA nicks (Cas9 nickase). | It can induce double-strand breaks in target DNA. | Induces DSBs in target DNA. | Li et al., 2013; Mao et al., 2013 |
| Off target effects | These effects can be minimized by selecting unique crRNA sequence. | These have off-target effects. | Off target effects cannot be avoided. | Hsu et al., 2013 |
| Generation of large scale libraries | YES, this is possible to generate large scale libraries. | Such generation is not possible because it requires customization of protein component for each gene. | Generation of large scale libraries is possible but technically difficult and challenging. | Cho et al., 2013; Hsu et al., 2013 |
| Protein engineering steps | It does not requires protein engineering steps, very simple to test multiple gRNA. | It requires complex to test gRNA. | TALENs need protein engineering steps to test gRNA. | Cho et al., 2013 |
| Cloning | Cloning is not necessary. | Cloning is necessary. | It requires cloning. | Cho et al., 2013 |
| gRNA production | Any number of gRNA can be produced by in vitro transcription. It keeps budget away from extra load. | Bit difficult to produce this kind of RNA. | gRNA production is bit difficult to achieve through these effector nucleases. | Cho et al., 2013 |
| Methylated DNA cleavage | It can cleave methylated DNA in human cells. This aspect is of special concern for plants as this has not been much explored | Unable to do so. | There are many question marks upon capacity of TALENs to perform methylated DNA cleavage. | Hsu et al., 2013; Ding et al., 2013 |
| Multiplexing | This is main advantage of CRISPR. Several genes can be edited at same time. Only Cas9 needed | Highly difficult to achieve this through ZFNs. | Very difficult to obtain multiplexed genes by means of TALENs. Because it needs separate dimeric proteins specific for each target | Li et al., 2013; Mao et al., 2013 |
| Structural proteins | CRISP R consists of single monomeric protein and chimeric RNA. | ZFNs work as dimeric and only protein component required. | TALENs also work as dimeric and require protein component. | Li et al., 2013; Upadhyay et al., 2013; Zhou et al., 2014 |
| Catalytic domain | It has two cleavage domains called RUVC and HNH. | ZFNs have catalytic domain of restriction endonuclease FOKI which generates a DSB. | TALENs also have FOKI catalytic domain of restriction endonuclease for DSB generation. | Jinek et al., 2012 |
| Mutation rate | Comparatively low mutation rate has been observed. | High mutation rate observed in plants. | Mutation rate is high as compared to CRISPR. | Li et al., 2013 |
| Components | crRNA, Cas9 proteins | Zn-finger domains Non-specific FokI nuclease domain | Zn-finger domains Non-specific FokI nuclease domain | Kumar and Jain, 2014 |
| Length of target sequence (bp) | 20–22 | 18–24 | 24–59 | Chen et al., 2016 |
| Target recognition efficiency | High | High | High | Kumar and Jain, 2014 |
| Level of experiment setup | Easy and very fast procedure of designing for new target site | Complicated procedure of redesigning for each new target site and need for expertise in protein engineering | Relatively easy procedure of designing for each new target site | Kumar and Jain, 2014 |