Sandbox Z-DNA

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Z-DNA Show:Asymmetric Unit Biological Assembly Drag the structure with the mouse to rotate   Export Animated Image

Z-DNA is a form of DNA that has a different structure from the more common form.It is a left-handed double helix wherein the sugar-phosphate backbone has a zigzag pattern due to the alternate stacking of bases in anti-conformation and syn conformation. In Z-DNA only a minor groove is present and the major groove is absent. The residues that allow sequence-specific recognition of Z-DNA are present on the convex outer surface.^[1] Z-DNA is thought play a role in regulation of gene expression, DNA processing events and/or genetic instability.^[2]

Contents 1 Structure 2 Z-DNA binding proteins 2.1 Double Stranded RNA adenosine deaminase 1, ADAR1 2.2 Vaccinia virus E3L protein 2.3 DLM-1 3 Movie Depicting ADAR1 binding to Z-DNA 4 Comparison of the three helices and helical parameters of DNA 5 References

Structure

B-Z DNA Show:Asymmetric Unit Biological Assembly Drag the structure with the mouse to rotate   Export Animated Image

Z-DNA can form invitro from B-DNA by raising negative super helical stress or under low salt conditions when deoxycytosine is 5-methylated. The formation of Z-DNA invivo is an energy requiring process. it forms behind a moving RNA polymerase when it moves through DNA double helix during transcription and is subsequently stabilized due to the generation of negative supercoils. Z-DNA is the first single crystal X-ray structure of a DNA fragment. It was crystallized as a self complementary DNA hexamer d(CG)₃ by Andrew Wang, Alexander Rich and their co-workers at MIT in 1979. ^[1][2]

Whenever B-DNA transforms into Z-DNA two form. The crystal structure of these junctions revealed, and at the junction. A crucial finding from this structure is that a right handed DNA can transform to a left handed DNA or vice versa by the disruption and extrusion of a base pair. It has also been suggested that the extruded base pairs at B-Z DNA junction may be sites for DNA modification.^[3]

Z-DNA binding proteins

Z-ALPHA and Z-DNA complex Show:Asymmetric Unit Biological Assembly Drag the structure with the mouse to rotate   Export Animated Image

Double Stranded RNA adenosine deaminase 1, ADAR1

ADAR1 belongs to the family of deaminases that modify double stranded mRNA by catalyzing the conversion of adenine to inosine which is then translated to guanosine. It is a complex protein with two Z-DNA binding motifs called and Z-beta.^[2] ADAR1 also has three copies of double-stranded RNA binding motif (DRBM) and a catalytic domain related to E.coli cytidine deaminase. The binding motif Z-alpha belongs to winged-helix-turn-helix family of proteins. It consists of a which has two alpha helices ( and ) connected by a short strand of amino acids and a . The beta sheet constrains the the fold by contacting the residues between alpha-2 and alpha-3.

The contact surface between consists of residues from the helix alpha-3 and COOH-terminal beta hairpin. Hydrogen bonding is present between Lys¹⁶⁹, Lys ¹⁷⁰, Asn¹⁷³, Arg¹⁷⁴ and Tyr¹⁷⁷ in the helix alpha-3 and . Lys¹⁶⁹, Asn¹⁷³, Arg¹⁷⁴, Trp¹⁹⁵ make water mediated phosphate contacts with Z-DNA. In addition Thr¹⁹¹ and Arg¹⁷⁴ of G2 and G6 on Z-DNA. An important interaction is the between aromatic ring of Tyr¹⁷⁷ and the carbon 8 of G4. This is unique to Z-DNA as the interaction requires the base to be in syn conformation. Pro¹⁹², Pro ¹⁹³ form another set of with Z-DNA where the pyrrolidine rings bond with the sugar-phosphate backbone from phosphate 2 to phosphate 3. Pro¹⁹² is conserved in Z-alpha and its homologues and forms a cis peptide bond which positions beta loop against the Z-DNA surface. ^[4]

The double stranded RNA substrate for ADAR1 is formed by folding of 3' intron back onto the exon containing the site to be edited. This shows that the editing of RNA occurs before the splicing of RNA providing an explanation for the binding of Z-DNA by ADAR1. Z-DNA may localize the editing activity of ADAR1 to a particular region within a gene, thus preventing indiscriminate modification. This allows for editing of the nascent transcript and blocking further transcription of gene. It has also been suggested that the extent of adenosine to inosine is proportional to amount of Z-DNA and also the ease with which the surrounding sequences adopt Z-DNA conformation. According to a study binding of ADAR1 to Z-DNA resulted in the increase in promoter activity of the gene which suggests that Z-DNA formation in the promoter region is itself involved in the regulation of transcription.^[1]

Vaccinia virus E3L protein

E3L protein of vaccinia virus acts as an immune modulator and is required for replication of the virus. The region of E3L is similar to the Z-alpha domain of ADAR1 but has a lower binding affinity to Z-DNA than ADAR1 or DLM-1. Though the C-terminal of E3L is sufficient for viral replication it is the N-terminal which is responsible for pathogenicity. Mutations or deletions in the N-terminal region reduces the pathogenicity of the virus. Replacement of this domain with its corresponding analogues from ADAR1 or DLM-1 generates a chimeric virus which is as lethal as the wild type virus. Thus a drug which can block the binding of E3L to Z-DNA may be an effective therapy in preventing pathogenicity. Similarity of E3L to variola also suggests that such drugs might be effective against small pox. ^[2][5] `

DLM-1

DLM-1 is also known as Z-DNA binding protein 1 (ZBP1). It is expressed by a tumor associated gene in lymphatic tissues and is upregulated in the peritoneal lining of mice with mouse ovarian ascites tumor. DLM-1 has two Z-DNA binding domains analogous to the Z-alpha and Z- beta domains in ADAR1. Comparison of Z-DNA binding of DLM-1 and ADAR1 revealed a common structure recognition core within the binding domain. However the role of DLM-1 binding to Z-DNA in tumor development is not known.

Z-DNA binding proteins have common structural characteristics. The binding domains of these proteins can substitute one another and thus can act as competitive inhibitors against one another. As explained above, disruption in the Z-DNA binding region of E3L reduces its pathogenicity. All these observations are important pointers towards the biological importance of Z-DNA.^[2]

Movie Depicting ADAR1 binding to Z-DNA

Comparison of the three helices and helical parameters of DNA

Sources^[6]

A-DNA Show:Asymmetric Unit Biological Assembly Drag the structure with the mouse to rotate   Export Animated Image

B-DNA Show:Asymmetric Unit Biological Assembly Drag the structure with the mouse to rotate   Export Animated Image

Z-DNA Show:Asymmetric Unit Biological Assembly Drag the structure with the mouse to rotate   Export Animated Image

Parameter	A-DNA	B-DNA	Z-DNA
Helix sense	right-handed	right-handed	left-handed
Residues per turn	11	10.5	12
Axial rise [Å]	2.55	3.4	3.7
Helix pitch(°)	28	34	45
Base pair tilt(°)	20	−6	7
Rotation per residue (°)	33	36	-30
Diameter of helix [Å]	23	20	18
Glycosidic bond configuration dA,dT,dC dG	anti anti	anti anti	anti syn
Sugar pucker dA,dT,dC dG	C3'-endo C3'-endo	C2'-endo C2'-endo	C2'-endo C3'-endo
Intrastrand phosphate-phosphate distance [Å] dA,dT,dC dG	5.9 5.9	7.0 7.0	7.0 5.9
Sources:[7][8][9]

References

1. ↑ ^{1.0 1.1 1.2} Rich A, Zhang S. Timeline: Z-DNA: the long road to biological function. Nat Rev Genet. 2003 Jul;4(7):566-72. PMID:12838348 doi:10.1038/nrg1115
2. ↑ ^{2.0 2.1 2.2 2.3 2.4} Wang G, Vasquez KM. Z-DNA, an active element in the genome. Front Biosci. 2007 May 1;12:4424-38. PMID:17485386
3. ↑ Ha SC, Lowenhaupt K, Rich A, Kim YG, Kim KK. Crystal structure of a junction between B-DNA and Z-DNA reveals two extruded bases. Nature. 2005 Oct 20;437(7062):1183-6. PMID:16237447 doi:10.1038/nature04088
4. ↑ Schwartz T, Rould MA, Lowenhaupt K, Herbert A, Rich A. Crystal structure of the Zalpha domain of the human editing enzyme ADAR1 bound to left-handed Z-DNA. Science. 1999 Jun 11;284(5421):1841-5. PMID:10364558
5. ↑ Kim YG, Lowenhaupt K, Oh DB, Kim KK, Rich A. Evidence that vaccinia virulence factor E3L binds to Z-DNA in vivo: Implications for development of a therapy for poxvirus infection. Proc Natl Acad Sci U S A. 2004 Feb 10;101(6):1514-8. Epub 2004 Feb 2. PMID:14757814 doi:10.1073/pnas.0308260100
6. ↑ van Dijk M, Bonvin AM. 3D-DART: a DNA structure modelling server. Nucleic Acids Res. 2009 Jul 1;37(Web Server issue):W235-9. Epub 2009 May, 5. PMID:19417072 doi:10.1093/nar/gkp287
7. ↑ Rich A, Nordheim A, Wang AH. The chemistry and biology of left-handed Z-DNA. Annu Rev Biochem. 1984;53:791-846. PMID:6383204 doi:http://dx.doi.org/10.1146/annurev.bi.53.070184.004043
8. ↑ Wang AH, Quigley GJ, Kolpak FJ, Crawford JL, van Boom JH, van der Marel G, Rich A. Molecular structure of a left-handed double helical DNA fragment at atomic resolution. Nature. 1979 Dec 13;282(5740):680-6. PMID:514347
9. ↑ Sinden, Richard R (1994-01-15). DNA structure and function (1st ed.). Academic Press. pp. 398. ISBN 0-12-645750-6.