Biology:Zinc-finger nuclease
Zinc-finger nucleases (ZFNs) are artificial restriction enzymes generated by fusing a zinc finger DNA-binding domain to a DNA-cleavage domain. Zinc finger domains can be engineered to target specific desired DNA sequences and this enables zinc-finger nucleases to target unique sequences within complex genomes. By taking advantage of endogenous DNA repair machinery, these reagents can be used to precisely alter the genomes of higher organisms. Alongside CRISPR/Cas9 and TALEN, ZFN is a prominent tool in the field of genome editing.
Domains
DNA-binding domain
The DNA-binding domains of individual ZFNs typically contain between three and six individual zinc finger repeats and can each recognize between 9 and 18 basepairs. If the zinc finger domains perfectly recognize a 3 basepair DNA sequence, they can generate a 3-finger array that can recognize a 9 basepair target site. Other procedures can utilize either 1-finger or 2-finger modules to generate zinc-finger arrays with six or more individual zinc fingers. The main drawback with this procedure is the specificities of individual zinc fingers can overlap and can depend on the context of the surrounding zinc fingers and DNA. Without methods to account for this "context dependence", the standard modular assembly procedure often fails.[1]
Numerous selection methods have been used to generate zinc-finger arrays capable of targeting desired sequences. Initial selection efforts utilized phage display to select proteins that bound a given DNA target from a large pool of partially randomized zinc-finger arrays. More recent efforts have utilized yeast one-hybrid systems, bacterial one-hybrid and two-hybrid systems, and mammalian cells. A promising new method to select novel zinc-finger arrays utilizes a bacterial two-hybrid system and has been dubbed "OPEN" by its creators.[2] This system combines pre-selected pools of individual zinc fingers that were each selected to bind a given triplet and then utilizes a second round of selection to obtain 3-finger arrays capable of binding a desired 9-bp sequence. This system was developed by the Zinc-Finger Consortium as an alternative to commercial sources of engineered zinc-finger arrays.
(see: Zinc finger chimera for more info on zinc finger selection techniques)
DNA-cleavage domain
The non-specific cleavage domain from the type IIs restriction endonuclease FokI is typically used as the cleavage domain in ZFNs.[4] This cleavage domain must dimerize in order to cleave DNA[5] and thus a pair of ZFNs are required to target non-palindromic DNA sites. Standard ZFNs fuse the cleavage domain to the C-terminus of each zinc finger domain. To let the two cleavage domains dimerize and cleave DNA, the two individual ZFNs must bind opposite strands of DNA with their C-termini a certain distance apart. The most commonly used linker sequences between the zinc finger domain and the cleavage domain requires the 5′ edge of each binding site to be separated by 5 to 7 bp.[6]
Several different protein engineering techniques have been employed to improve both the activity and specificity of the nuclease domain used in ZFNs. Directed evolution has been employed to generate a FokI variant with enhanced cleavage activity that the authors dubbed "Sharkey".[7] Structure-based design has also been employed to improve the cleavage specificity of FokI by modifying the dimerization interface so that only the intended heterodimeric species are active.[8][9][10][11]
Applications
Zinc finger nucleases are useful to manipulate the genomes of many plants and animals including arabidopsis,[12][13] tobacco,[14][15] soybean,[16] corn,[17] Drosophila melanogaster,[18] C. elegans,[19] Platynereis dumerilii,[20] sea urchin,[21] silkworm,[22] zebrafish,[23] frogs,[24] mice,[25] rats,[26] rabbits,[27] pigs,[28] cattle,[29] and various types of mammalian cells.[30] Zinc finger nucleases have also been used in a mouse model of haemophilia[31] and a clinical trial found CD4+ human T-cells with the CCR5 gene disrupted by zinc finger nucleases to be safe as a potential treatment for HIV/AIDS.[32] ZFNs are also used to create a new generation of genetic disease models called isogenic human disease models.
Disabling an allele
ZFNs can be used to disable dominant mutations in heterozygous individuals by producing double-strand breaks (DSBs) in the DNA (see Genetic recombination) in the mutant allele, which will, in the absence of a homologous template, be repaired by non-homologous end-joining (NHEJ). NHEJ repairs DSBs by joining the two ends together and usually produces no mutations, provided that the cut is clean and uncomplicated. In some instances, however, the repair is imperfect, resulting in deletion or insertion of base-pairs, producing frame-shift and preventing the production of the harmful protein.[33] Multiple pairs of ZFNs can also be used to completely remove entire large segments of genomic sequence.[34] To monitor the editing activity, a PCR of the target area amplifies both alleles and, if one contains an insertion, deletion, or mutation, it results in a heteroduplex single-strand bubble that cleavage assays can easily detect. ZFNs have also been used to modify disease-causing alleles in triplet repeat disorders. Expanded CAG/CTG repeat tracts are the genetic basis for more than a dozen inherited neurological disorders including Huntington's disease, myotonic dystrophy, and several spinocerebellar ataxias. It has been demonstrated in human cells that ZFNs can direct double-strand breaks (DSBs) to CAG repeats and shrink the repeat from long pathological lengths to short, less toxic lengths.[35]
Recently, a group of researchers have successfully applied the ZFN technology to genetically modify the gol pigment gene and the ntl gene in zebrafish embryo. Specific zinc-finger motifs were engineered to recognize distinct DNA sequences. The ZFN-encoding mRNA was injected into one-cell embryos and a high percentage of animals carried the desired mutations and phenotypes. Their research work demonstrated that ZFNs can specifically and efficiently create heritable mutant alleles at loci of interest in the germ line, and ZFN-induced alleles can be propagated in subsequent generations.
Similar research of using ZFNs to create specific mutations in zebrafish embryo has also been carried out by other research groups. The kdr gene in zebra fish encodes for the vascular endothelial growth factor-2 receptor. Mutagenic lesions at this target site was induced using ZFN technique by a group of researchers in US. They suggested that the ZFN technique allows straightforward generation of a targeted allelic series of mutants; it does not rely on the existence of species-specific embryonic stem cell lines and is applicable to other vertebrates, especially those whose embryos are easily available; finally, it is also feasible to achieve targeted knock-ins in zebrafish, therefore it is possible to create human disease models that are heretofore inaccessible.
Allele editing
ZFNs are also used to rewrite the sequence of an allele by invoking the homologous recombination (HR) machinery to repair the DSB using the supplied DNA fragment as a template. The HR machinery searches for homology between the damaged chromosome and the extra-chromosomal fragment and copies the sequence of the fragment between the two broken ends of the chromosome, regardless of whether the fragment contains the original sequence. If the subject is homozygous for the target allele, the efficiency of the technique is reduced since the undamaged copy of the allele may be used as a template for repair instead of the supplied fragment.
Gene therapy
The success of gene therapy depends on the efficient insertion of therapeutic genes at an appropriate chromosomal target site within the human genome, without causing cell injury, oncogenic mutations, or an immune response. The construction of plasmid vectors is simple and straightforward. Custom-designed ZFNs that combine the non-specific cleavage domain (N) of FokI endonuclease with zinc-finger proteins (ZFPs) offer a general way to deliver a site-specific DSB to the genome, and stimulate local homologous recombination by several orders of magnitude. This makes targeted gene correction or genome editing a viable option in human cells. Since ZFN-encoding plasmids could be used to transiently express ZFNs to target a DSB to a specific gene locus in human cells, they offer an excellent way for targeted delivery of the therapeutic genes to a pre-selected chromosomal site. The ZFN-encoding plasmid-based approach has the potential to circumvent all the problems associated with the viral delivery of therapeutic genes.[36] The first therapeutic applications of ZFNs are likely to involve ex vivo therapy using a patient's own stem cells. After editing the stem cell genome, the cells could be expanded in culture and reinserted into the patient to produce differentiated cells with corrected functions. Initial targets likely include the causes of monogenic diseases, such as the IL2Rγ gene and the β-globin gene for gene correction and CCR5 gene for mutagenesis and disablement.[33]
Potential problems
Off-target cleavage
If the zinc finger domains are not specific enough for their target site or they do not target a unique site within the genome of interest, off-target cleavage may occur. Such off-target cleavage may lead to the production of enough double-strand breaks to overwhelm the repair machinery and, as a consequence, yield chromosomal rearrangements and/or cell death. Off-target cleavage events may also promote random integration of donor DNA.[33] Two separate methods have been demonstrated to decrease off-target cleavage for 3-finger ZFNs that target two adjacent 9-basepair sites.[37] Other groups use ZFNs with 4, 5 or 6 zinc fingers that target longer and presumably rarer sites and such ZFNs could theoretically yield less off-target activity. A comparison of a pair of 3-finger ZFNs and a pair of 4-finger ZFNs detected off-target cleavage in human cells at 31 loci for the 3-finger ZFNs and at 9 loci for the 4-finger ZFNs.[38] Whole genome sequencing of C. elegans modified with a pair of 5-finger ZFNs found only the intended modification and a deletion at a site "unrelated to the ZFN site" indicating this pair of ZFNs was capable of targeting a unique site in the C. elegans genome.[19]
Immunogenicity
As with many foreign proteins inserted into the human body, there is a risk of an immunological response against the therapeutic agent and the cells in which it is active. Since the protein must be expressed only transiently, however, the time over which a response may develop is short.[33]
Liu et al. respectively target ZFNickases to the endogenous b-casein(CSN2) locus stimulates lysostaphin and human lysozyme gene addition by homology-directed repair and derive secrete lysostaphin cows.[39][40]
Prospects
The ability to precisely manipulate the genomes of plants and animals has numerous applications in basic research, agriculture, and human therapeutics. Using ZFNs to modify endogenous genes has traditionally been a difficult task due mainly to the challenge of generating zinc finger domains that target the desired sequence with sufficient specificity. Improved methods of engineering zinc finger domains and the availability of ZFNs from a commercial supplier now put this technology in the hands of increasing numbers of researchers. Several groups are also developing other types of engineered nucleases including engineered homing endonucleases[41] [42] and nucleases based on engineered TAL effectors.[43][44] TAL effector nucleases (TALENs) are particularly interesting because TAL effectors appear to be very simple to engineer[45] [46] and TALENs can be used to target endogenous loci in human cells.[47] But to date no one has reported the isolation of clonal cell lines or transgenic organisms using such reagents. One type of ZFN, known as SB-728-T, has been tested for potential application in the treatment of HIV.[48]
Zinc-finger nickases
Zinc-finger nickases (ZFNickases) are created by inactivating the catalytic activity of one ZFN monomer in the ZFN dimer required for double-strand cleavage.[49] ZFNickases demonstrate strand-specific nicking activity in vitro and thus provide for highly specific single-strand breaks in DNA.[49] These SSBs undergo the same cellular mechanisms for DNA that ZFNs exploit, but they show a significantly reduced frequency of mutagenic NHEJ repairs at their target nicking site. This reduction provides a bias for HR-mediated gene modifications. ZFNickases can induce targeted HR in cultured human and livestock cells, although at lower levels than corresponding ZFNs from which they were derived because nicks can be repaired without genetic alteration.[39][50] A major limitation of ZFN-mediated gene modifications is the competition between NHEJ and HR repair pathways. Regardless of the presence of a DNA donor construct, both repair mechanisms can be activated following DSBs induced by ZFNs. Thus, ZFNickases is the first plausible attempt at engineering a method to favor the HR method of DNA repair as opposed to the error-prone NHEJ repair. By reducing NHEJ repairs, ZFNickases can thereby reduce the spectrum of unwanted off-target alterations. The ease by which ZFNickases can be derive from ZFNs provides a great platform for further studies regarding the optimization of ZFNickases and possibly increasing their levels of targeted HR while still maintain their reduced NHEJ frequency.
See also
- Chimeric nuclease
- Genome editing
- Gene targeting
- Zinc finger protein
- Zinc finger chimera
- Protein engineering
- Zinc finger nuclease treatment of HIV
- CompoZr
References
- ↑ "Unexpected failure rates for modular assembly of engineered zinc fingers". Nat. Methods 5 (5): 374–375. May 2008. doi:10.1038/nmeth0508-374. PMID 18446154.
- ↑ "Rapid "open-source" engineering of customized zinc-finger nucleases for highly efficient gene modification". Mol. Cell 31 (2): 294–301. September 2008. doi:10.1016/j.molcel.2008.06.016. PMID 18657511.
- ↑ "Genome engineering with zinc-finger nucleases". Genetics 188 (4): 773–782. 2011. doi:10.1534/genetics.111.131433. PMID 21828278.
- ↑ "Hybrid restriction enzymes: zinc finger fusions to Fok I cleavage domain". Proc Natl Acad Sci USA 93 (3): 1156–1160. 1996. doi:10.1073/pnas.93.3.1156. PMID 8577732. Bibcode: 1996PNAS...93.1156K.
- ↑ "FokI dimerization is required for DNA cleavage". Proc Natl Acad Sci USA 95 (18): 10570–10575. 1998. doi:10.1073/pnas.95.18.10570. PMID 9724744. Bibcode: 1998PNAS...9510570B.
- ↑ "Zinc-finger nucleases: the next generation emerges". Mol. Ther. 16 (7): 1200–1207. July 2008. doi:10.1038/mt.2008.114. PMID 18545224.
- ↑ "Directed Evolution of an Enhanced and Highly Efficient FokI Cleavage Domain for Zinc Finger Nucleases". Journal of Molecular Biology 400 (1): 96–107. 2010. doi:10.1016/j.jmb.2010.04.060. PMID 20447404.
- ↑ "Structure-based redesign of the dimerization interface reduces the toxicity of zinc-finger nucleases". Nature Biotechnology 25 (7): 786–793. 2007. doi:10.1038/nbt1317. PMID 17603476. http://www.escholarship.org/uc/item/52x577fp.
- ↑ "An improved zinc-finger nuclease architecture for highly specific genome editing". Nature Biotechnology 25 (7): 778–785. 2007. doi:10.1038/nbt1319. PMID 17603475.
- ↑ "Enhancing zinc-finger-nuclease activity with improved obligate heterodimeric architectures". Nature Methods 8 (1): 74–79. 2010. doi:10.1038/nmeth.1539. PMID 21131970.
- ↑ "Creating Designed Zinc-Finger Nucleases with Minimal Cytotoxicity". Journal of Molecular Biology 405 (3): 630–641. 2011. doi:10.1016/j.jmb.2010.10.043. PMID 21094162.
- ↑ "High frequency targeted mutagenesis in Arabidopsis thaliana using zinc finger nucleases". Proceedings of the National Academy of Sciences 107 (26): 12028–12033. 2010. doi:10.1073/pnas.0914991107. PMID 20508152. Bibcode: 2010PNAS..10712028Z.
- ↑ "Site-directed mutagenesis in Arabidopsis using custom-designed zinc finger nucleases". Proceedings of the National Academy of Sciences 107 (26): 12034–12039. 2010. doi:10.1073/pnas.1000234107. PMID 20508151. Bibcode: 2010PNAS..10712034O.
- ↑ "Targeted transgene integration in plant cells using designed zinc finger nucleases". Plant Molecular Biology 69 (6): 699–709. 2008. doi:10.1007/s11103-008-9449-7. ISSN 0167-4412. PMID 19112554.
- ↑ "High-frequency modification of plant genes using engineered zinc-finger nucleases". Nature 459 (7245): 442–445. 2009. doi:10.1038/nature07845. PMID 19404258. Bibcode: 2009Natur.459..442T.
- ↑ "Targeted Mutagenesis of Duplicated Genes in Soybean with Zinc-Finger Nucleases". Plant Physiology 156 (2): 466–473. 2011. doi:10.1104/pp.111.172981. PMID 21464476.
- ↑ "Precise genome modification in the crop species Zea mays using zinc-finger nucleases". Nature 459 (7245): 437–441. May 2009. doi:10.1038/nature07992. PMID 19404259. Bibcode: 2009Natur.459..437S.
- ↑ "Enhancing Gene Targeting with Designed Zinc Finger Nucleases". Science 300 (5620): 764. 2003. doi:10.1126/science.1079512. PMID 12730594.
- ↑ 19.0 19.1 "Targeted Genome Editing Across Species Using ZFNs and TALENs". Science 333 (6040): 307. 2011. doi:10.1126/science.1207773. PMID 21700836. Bibcode: 2011Sci...333..307W.
- ↑ "Spectral Tuning of Phototaxis by a Go-Opsin in the Rhabdomeric Eyes of Platynereis". Current Biology 25 (17): 2265–2271. August 2015. doi:10.1016/j.cub.2015.07.017. PMID 26255845.
- ↑ "Targeted mutagenesis in the sea urchin embryo using zinc-finger nucleases". Genes to Cells 15 (8): 875–885. 2010. doi:10.1111/j.1365-2443.2010.01425.x. PMID 20604805. http://ir.lib.hiroshima-u.ac.jp/00033718.
- ↑ "Targeted mutagenesis in the silkworm Bombyx mori using zinc finger nuclease mRNA injection". Insect Biochemistry and Molecular Biology 40 (10): 759–765. 2010. doi:10.1016/j.ibmb.2010.07.012. PMID 20692340.
- ↑ "Zinc Finger–Based Knockout Punches for Zebrafish Genes". Zebrafish 5 (2): 1121–1123. 2008. doi:10.1089/zeb.2008.9988. PMID 18554175.
- ↑ "Efficient targeted gene disruption in the soma and germ line of the frog Xenopus tropicalis using engineered zinc-finger nucleases". Proceedings of the National Academy of Sciences 108 (17): 7052–7057. 2011. doi:10.1073/pnas.1102030108. PMID 21471457. Bibcode: 2011PNAS..108.7052Y.
- ↑ "Distinct Factors Control Histone Variant H3.3 Localization at Specific Genomic Regions". Cell 140 (5): 678–691. 2010. doi:10.1016/j.cell.2010.01.003. PMID 20211137.
- ↑ "Knockout Rats via Embryo Microinjection of Zinc-Finger Nucleases". Science 325 (5939): 433. 2009. doi:10.1126/science.1172447. PMID 19628861. Bibcode: 2009Sci...325..433G.
- ↑ "Efficient Immunoglobulin Gene Disruption and Targeted Replacement in Rabbit Using Zinc Finger Nucleases". PLOS ONE 6 (6): e21045. 2011. doi:10.1371/journal.pone.0021045. PMID 21695153. Bibcode: 2011PLoSO...621045F.
- ↑ "Efficient generation of a biallelic knockout in pigs using zinc-finger nucleases". Proceedings of the National Academy of Sciences 108 (29): 12013–12017. 2011. doi:10.1073/pnas.1106422108. PMID 21730124. Bibcode: 2011PNAS..10812013H.
- ↑ "Highly efficient modification of beta-lactoglobulin (BLG) gene via zinc-finger nucleases in cattle". Cell Research 21 (11): 1638–1640. 2011. doi:10.1038/cr.2011.153. PMID 21912434.
- ↑ "Zinc-finger Nucleases as Gene Therapy Agents". Gene Therapy 15 (22): 1463–1468. 2008. doi:10.1038/gt.2008.145. PMID 18784746.
- ↑ "In vivo genome editing restores haemostasis in a mouse model of haemophilia". Nature 475 (7355): 217–221. 2011. doi:10.1038/nature10177. PMID 21706032.
- ↑ "Gene Editing of CCR5 in Autologous CD4 T Cells of Persons Infected with HIV". New England Journal of Medicine 370 (10): 901–910. 6 March 2014. doi:10.1056/NEJMoa1300662. PMID 24597865.
- ↑ 33.0 33.1 33.2 33.3 "Zinc finger nucleases: custom-designed molecular scissors for genome engineering of plant and mammalian cells". Nucleic Acids Res. 33 (18): 5978–5990. 2005. doi:10.1093/nar/gki912. PMID 16251401.
- ↑ "Targeted chromosomal deletions in human cells using zinc finger nucleases". Genome Res. 20 (1): 81–89. December 2009. doi:10.1101/gr.099747.109. PMID 19952142.
- ↑ "Zinc-finger directed double-strand breaks within CAG repeat tracts promote repeat instability in human cells". Proceedings of the National Academy of Sciences of the United States of America 106 (24): 9607–9612. 16 June 2009. doi:10.1073/pnas.0902420106. PMID 19482946. Bibcode: 2009PNAS..106.9607M.
- ↑ "Plasmids for Gene Therapy". Plasmids: Current Research and Future Trends. Norfolk: Caister Academic Press. 2008. ISBN 978-1-904455-35-6.
- ↑ "Zinc finger protein-dependent and -independent contributions to the in vivo off-target activity of zinc finger nucleases". Nucleic Acids Res 39 (1): 381–392. September 2010. doi:10.1093/nar/gkq787. PMID 20843781.
- ↑ "Revealing Off-Target Cleavage Specificities of Zinc Finger Nucleases by in Vitro Selection". Nature Methods 8 (9): 765–770. 2011. doi:10.1038/nmeth.1670. PMID 21822273.
- ↑ 39.0 39.1 "Zinc-finger nickase-mediated insertion of the lysostaphin gene into the beta-casein locus in cloned cows". Nature Communications 4: 2565. 2013. doi:10.1038/ncomms3565. PMID 24121612. Bibcode: 2013NatCo...4.2565L.
- ↑ "Generation of mastitis resistance in cows by targeting human lysozyme gene to -casein locus using zinc-finger nucleases". Proceedings of the Royal Society B: Biological Sciences 281 (1780): 20133368. 2014. doi:10.1098/rspb.2013.3368. PMID 24552841.
- ↑ "Efficient targeting of a SCID gene by an engineered single-chain homing endonuclease". Nucleic Acids Res. 37 (16): 5405–5419. September 2009. doi:10.1093/nar/gkp548. PMID 19584299.
- ↑ "Heritable targeted mutagenesis in maize using a designed endonuclease". The Plant Journal 61 (1): 176–187. 2010. doi:10.1111/j.1365-313X.2009.04041.x. PMID 19811621.
- ↑ "Targeting DNA Double-Strand Breaks with TAL Effector Nucleases". Genetics 186 (2): 757–761. July 2010. doi:10.1534/genetics.110.120717. PMID 20660643.
- ↑ "TAL nucleases (TALNs): hybrid proteins composed of TAL effectors and FokI DNA-cleavage domain". Nucleic Acids Res 39 (1): 359–372. August 2010. doi:10.1093/nar/gkq704. PMID 20699274.
- ↑ "A simple cipher governs DNA recognition by TAL effectors". Science 326 (5959): 1501. December 2009. doi:10.1126/science.1178817. PMID 19933106. Bibcode: 2009Sci...326.1501M.
- ↑ "Breaking the code of DNA binding specificity of TAL-type III effectors". Science 326 (5959): 1509–1512. December 2009. doi:10.1126/science.1178811. PMID 19933107. Bibcode: 2009Sci...326.1509B.
- ↑ "A TALE nuclease architecture for efficient genome editing". Nature Biotechnology 29 (2): 143–148. 2010. doi:10.1038/nbt.1755. PMID 21179091.
- ↑ "Zinc Fingers Could Be Key to Reviving Gene Therapy". 28 December 2009. https://www.nytimes.com/2009/12/29/health/research/29zinc.html?_r=0.
- ↑ 49.0 49.1 "Engineered zinc finger nickases induce homology-directed repair with reduced mutagenic effects". Nucleic Acids Research 40 (7): 5560–5568. 2012. doi:10.1093/nar/gks179. PMID 22373919.
- ↑ "Targeted gene addition to a predetermined site in the human genome using a ZFN-based nicking enzyme". Genome Research 22 (4): 1316–1326. 2012. doi:10.1101/gr.122879.111. PMID 22434427.
Further reading
- "Zinc Finger Tools: custom DNA-binding domains for transcription factors and nucleases". Nucleic Acids Res. 34 (Web Server issue): W516–23. July 2006. doi:10.1093/nar/gkl209. PMID 16845061.
- "Gene targeting using zinc finger nucleases". Nat. Biotechnol. 23 (8): 967–973. August 2005. doi:10.1038/nbt1125. PMID 16082368.
- "Heritable Targeted Gene Disruption in Zebrafish Using Designed Zinc Finger Nucleases". Nat. Biotechnol. 26 (6): 702–708. June 2008. doi:10.1038/nbt1409. PMID 18500334.
- "Targeted gene inactivation in zebrafish using engineered zinc finger nucleases". Nat. Biotechnol. 26 (6): 695–701. June 2008. doi:10.1038/nbt1398. PMID 18500337.
External links
- Zinc finger selector
- Zinc Finger Consortium website
- Zinc Finger Consortium materials from Addgene
- A commercial supplier of ZFNs
Original source: https://en.wikipedia.org/wiki/Zinc-finger nuclease.
Read more |