Human bromodomain containing protein 2 (bromodomain 2) in complex with JQ1/SGCBD01 probe against BET subfamily

Target ID:

BRD2A

Deposition Date:

Tuesday 31st August 2010

Families:

Bromodomain

Related Diseases:

Cancer and epigenetics

Structure type:

protein-ligand

Download Coordinates:

3ONI

Authors:

Filippakopoulos, P., Picaud, S., Qi, J., Keates, T., Felletar, I., Fedorov, O., Muniz, J., von Delft, F., Arrowsmith, C.H., Edwards, A.M., Weigelt, J., Bountra, C., Bradner, J.E., Knapp, S.

Site:

Oxford

3ONI

tabs

Structure Details

BRD2 belongs to the BET subclass of proteins, which are distinguished by two N-terminal bromodomains and one ET (Extra Terminal) domain. BRDs have been found to be associated with chromatin. The poorly characterized ET domain functions as a protein-protein interaction motif and may be part of an atypical serine-kinase activity. The subclass consists of at least four members in mouse and human, Brd2 (also referred to as Fsrg1, RING3), Brd3 (Fsrg2, ORFX), Brd4 (Fsrg4, MCAP/HUNK1), and Brdt (Fsrg3, BRD6). BRD proteins are related to the female sterile homeotic protein gene in Drosophila, a gene required maternally for proper expression of other homeotic genes, such as Ubx, which is involved in pattern formation. BRD2- and BRD3 associated chromatin is significantly enriched in K5- and K12-acetylated histone H4. Importantly, BET-BRDs stay associated with chromatin during mitosis. This unique feature of the BET proteins is utilized by papilloma and Kaposi?s sarcoma-associated herpesviruses for tethering their genomes to the mitotic chromosome of their host, resulting in viral propagation during the cell division. BRD2 is ubiquitously expressed in mammalian tissues. Brd2 has been shown to bind to E2F proteins, but also co-activator TAFs, members of the SWI/SNF complex, HATs and HDACs (histone deacetylases) to regulate the expression of diverse genes. Brd2 can function either as a transcriptional co-activator or co-repressor, depending on the specific promoter and cellular context and has been shown to regulate the expression of cyclin A. Constitutive over-expression of Brd2 in the B-cells of transgenic mice results in the development of B-cell lymphoma and leukaemia. BRD2 knockout mice are embryonic lethal. Targeted disruption of the Brd2 gene in the promoter region, leading to the reduced expression of Brd2 produces a hypomorphic phenotype without gross developmental abnormalities. Interestingly, these mice are extreme obese with hyperinsulinaemia, pancreatic islet expansion, hepatosteatosis and elevated pro-inflammatory cytokines, but, surprisingly enhanced glucose tolerance and low blood glucose levels. In pre-adipocytes, Brd2 knockdown promotes adipogenic differentiation by enhancing PPAR-γ transcription. Here we present the structure of the second bromodomain with the BET-specific bromodomain inhibitor JQ1.

Materials and Methods

Entry Clone Source: in house ingeniering

Entry Clone Accession: n/a

SGC Construct ID: BRD2A-c013

GenBank GI number: gi|4826806

Vector: pNIC28-Bsa4. Details [PDF ]; Sequence [ FASTA ] or [ GenBank ]

Amplified construct sequence:
CATATGCACCATCATCATCATCATTC
TTCTGGTGTAGATCTGGGTACCGAGA
ACCTGTACTTCCAATCCATGGGCAAA
CTGAGCGAACAACTGAAGCATTGCAA
TGGCATTCTTAAAGAGCTCCTGAGTA
AAAAACACGCCGCCTATGCGTGGCCA
TTTTATAAACCGGTGGATGCCTCTGC
GCTGGGTCTGCATGATTATCACGATA
TCATTAAACATCCGATGGATCTCTCA
ACCGTTAAACGTAAAATGGAAAATCG
CGATTATCGTGATGCCCAGGAATTTG
CGGCGGATGTACGCCTCATGTTTTCG
AACTGCTACAAATATAACCCTCCAGA
TCACGATGTTGTGGCAATGGCACGAA
AGCTACAGGATGTATTTGAGTTCCGT
TATGCCAAGATGCCAGATTGACAGTA
AAGGTGGATACGGATCCGAA

Final protein sequence (Tag sequence in lowercase):
mhhhhhhssgvdlgtenlyfq^smGK
LSEQLKHCNGILKELLSKKHAAYAWP
FYKPVDASALGLHDYHDIIKHPMDLS
TVKRKMENRDYRDAQEFAADVRLMFS
NCYKYNPPDHDVVAMARKLQDVFEFR
YAKMPD

^ TEV cleavage site

Tags and additions: Cleavable N-terminal His6 tag.

Host: BL21 (DE3)R3-pRARE2 (Phage resistant strain).

Growth medium, induction protocol: 10 ml from a 50 ml overnight culture containing 50 µg/ml kanamycin and 34 µg/ml chloramphenicol were used to inoculate each of two 1 liter cultures of TB containing 50 µg/ml kanamycin and 34 µg/ml chloramphenicol. Cultures were grown at 37°C until the OD₆₀₀ reached ~2.5 then the temperature was adjusted to 18°C. Expression was induced overnight using 0.1 mM IPTG at an OD₆₀₀ of 3.0. The cells were collected by centrifugation and the pellet re-suspended in binding buffer and frozen.
Lysis buffer: 50 mM HEPES pH 7.5; 500 mM NaCl; 10 mM Imidazole, 5% Glycerol.
Extraction buffer, extraction method: Frozen pellets were thawed and fresh 0.5 mM TCEP, 1 mM PMSF added to the lysate. Cells were lysed using sonication. The lysate was centrifuged at 17,000rpm for 60 minutes and the supernatant collected for purification.

Column 1: Ni-affinity. Ni-sepharose (Amersham), 5ml of 50% slurry in 1.5 x 10cm column, washed with binding buffer.

Column 1 Buffer:
Binding buffer: 50 mM HEPES, pH 7.5; 500 mM NaCl; 5% glycerol; 5 mM imidazole.
Wash buffer: 50 mM HEPES, pH 7.5; 500 mM NaCl; 5% glycerol; 30 mM Imidazole.
Elution buffer: 50 mM HEPES, pH 7.5; 500 mM NaCl; 5% glycerol; 50 to 250 mM Imidazole(step elution).

Column 1 Procedure: The supernatant was loaded by gravity flow on the Ni-sepharose column. The column was then washed with 30ml wash buffer at gravity flow. The protein was eluted by gravity flow by applying 5ml portions of elution buffer with increasing concentration of imidazole (50 mM, 100 mM, 150 mM, 200 and 250 mM); fractions were collected until essentially all protein was eluted.

Enzymatic treatment: The N-terminal His tag was cleaved by treatment with TEV protease, overnight.

Column 2: Size Exclusion Chromatography. Superdex S75 16/60 HiLoad.

Column 2 Buffers: 10 mM HEPES, pH 7.5; 500 mM NaCl; 5% glycerol.

Column 2 Procedure: The protein was concentrated and applied to an S75 16/60 HiLoad gel filtration column equilibrated in 10 mM HEPES, pH 7.5; 500 mM NaCl; 5% glycerol using an ÄKTA express system.

Mass spectrometry characterization: LC- ESI -MS TOF gave a measured mass of 13351Da for this construct as predicted from the sequence of this protein.

Protein concentration: Protein was concentrated to 8.2mg/ml using an Amicon 3kDa cut-off concentrator.

Crystallisation: Crystals were grown at 4°C in 150nl sitting drops from a 2:1 ratio of a protein solution (11.2mg/ml) to reservoir solution containing 30% Jeffamine 600, 0.05 M CsCl, 0.1 M MES pH 6.5.

Data Collection: Crystals were cryo-protected using the well solution supplemented by 20% ethylene glycol and flash frozen in liquid nitrogen.
X-ray source: Diffraction data were collected from a single crystal on a Rigaku FRE at a single wavelength of 1.54 Å. The final structure was refined to 1.61 Å.
Phasing: The structure was solved by molecular replacement using an ensemble of known bromodomain structure as a starting model.

References

LeRoy G, Rickards B, Flint SJ. The double bromodomain proteins Brd2 and Brd3 couple histone acety
Nakamura Y, Umehara T, Nakano K, Jang MK, Shirouzu M, Morita S, Uda-Tochio H, Hamana H, Terada T, Adachi N, et al. Crystal structure of the human BRD2 bromodomain: insights into dimerization and recognition of acetylated histone H4. J Biol Chem. 2007;282:4193?4201.
Denis GV, Vaziri C, Guo N, Faller DV. RING3 kinase transactivates promoters of cell cycle regulatory genes through E2F. Cell Growth Differ. 2000;11:417?424.
Wang F, Liu H, Blanton WP, Belkina A, Lebrasseur NK, Denis GV. Brd2 disruption in mice causes severe obesity without Type 2 diabetes. Biochem J. 2009; 425(1):71-83.
Shang E, Wang X, Wen D, Greenberg DA, Wolgemuth DJ. Double bromodomain-containing gene Brd2 is essential for embryonic development in mouse. Dev Dyn. 2009;238(4): 908-917.
Panagis Filippakopoulos, Jun Qi, Sarah Picaud, Yao Shen, William B. Smith, Tracey Keates, Elizabeth M. Morse, Oleg Fedorov, Tyler T. Hickman, Ildiko Felletar, Martin Philpott, Shonagh Munro, Nathan West, Michael J. Cameron, Tom Heightman, Nicholas LaThangue, Andrew Kung, Christopher A. French, Olaf Wiest, Stefan Knapp, James E. Bradner. (2010).. Selective inhibition of BET bromodomains. Nature; 468(7327):1067-1073.