Robert E. Kingston (born in 1954) is an American biochemist and geneticist who studies the functional and regulatory role nucleosomes play in gene expression, specifically during early development.[1] After receiving his PhD (1981) and completing post-doctoral research, Kingston became an assistant professor at Massachusetts General Hospital (1985), where he started a research laboratory focused on understanding chromatin's structure with regards to transcriptional regulation.[1] As a Harvard graduate himself, Kingston has served his alma mater through his leadership.[1]
Robert E. Kingston | |
---|---|
Alma mater | Harvard College, University of California, Berkeley |
Known for | Nucleosome biology |
Scientific career | |
Institutions | Massachusetts General Hospital |
Doctoral advisor | Michael Chamberlin |
Other academic advisors | Phillip Sharp |
Notable students | Geeta Narlikar |
He was the head of the Harvard's Biological and Biomedical Sciences PhD program from 2004 to 2007, the chair of the molecular biology department at Massachusetts General Hospital from 2005 to 2023, the vice-chair of the department of genetics at Harvard Medical School, and the chair of the executive committee on research at Massachusetts General Hospital from 2012 to 2015. [2][1] In November 2022, he was appointed as the inaugural Chief Academic Officer and Senior Vice President for Research and Education for Massachusetts General Hospital effective January 2023.[3]
In addition to being a professor of genetics at Harvard Medical School, Kingston frequently organizes conferences and performs editorials on his research interests.[1] In 2016, he was elected by his peers to be a member of the National Academy of Sciences.[2]
Education
editKingston graduated from Harvard College in 1976.[1] Four years later, he completed his PhD on bacterial regulatory mechanisms at the University of California, Berkeley, while under the mentorship of Michael Chamberlin.[1] He then performed postdoctoral research on mammalian post-transcriptional mechanisms at the Massachusetts Institute of Technology under the supervision of Dr. Philip Sharp.[1]
Research
editKingston's research continues to have a significant impact on developmental biology and epigenetics, as it focuses on an important feature of eukaryotic gene expression: chromatin remodeling.[2] His research can be applied to the field of gene therapy, specifically principles surrounding chromatin regulation.[2]
nusA protein
editIn 1981, Kingston received his PhD after working on a number of research initiatives surrounding genome regulation and expression. Through an in vitro study that mapped termination sites dependent on the nusA protein, he discovered that in vivo rRNA transcription is regulated by turnstile attenuation, a mechanism that terminates rrnB chains in the leader region.[4] He found that this happens because of the specific presence and location of pause sites, located 90 and 91 bases from the P1 promoter, which are sensitive to the presence of nusA protein and concentration of regulatory nucleotide guanosine tetraphosphate.[4]
Heat shock protein 70 (HSP70)
editAfter recognizing that the myc gene was involved with tumor formation, Kingston drew a parallel between the presence of the myc gene and the increased genomic expression of HSP70.[5] He also found that the genomic expression of HSP70 is also dependent on physiological stresses.5 Analyzing the gene sequences showed that heat shock, cadmium induction, and metallothionein II responsiveness are needed for HSP70 gene expression during the primary level of transcription.[6] He observed that while the physiological factors have a role on one domain (distal) of the HSP70 promoter, the other domain (proximal) is more responsive to serum stimulation.[6] After conducting in vitro transcription experiments, Kingston found that there is a heat-shock transcription factor (HSTF) that allows the interactions with the heat shock element (HSE), and that the HSP70 gene promoter also depends on a CCAAT-box-binding transcription factor (CTF) for CCAAT-box-dependent transcription.[7] In vitro cell-free systems that have heat-induced activation of human heat-shock factor (HSF) were used to determine that at 43 °C, HSF undergoes post-translational modification to where it can then bind to a specific DNA sequence, HSE.[8]
SWI/SNF subunits of chromatin remodeling
editKingston's primary research interests surround chromatin remodeling, and his breakthroughs within the field began when he discovered the functional subunit responsibilities of SWI/SNF, a chromatin remodeling complex that causes specific transcription factors to bind to nucleosomal DNA.[9] He defined that two SWI/SNF subunits, BRG1 and BAF155, along with EKLF zinc-finger DNA binding domains (DBDs) can be used to remodel chromatin, meaning that these specific domains of SWI/SNF have an effect on transcription factor-directed nucleosome remodeling.[9] He was also able to conclude that different domains of transcription factors target SWI/SNF complexes to chromatin in a gene-selective way.[9] His work on nucleosomal DNA extends to his findings on TATA-binding protein (TPB), specifically how dynamic remodeling of chromatin can allow for TPB to bind onto the TATA sequence. His work on SWI/SNF led him to conclude that these two subunits are responsible for an “activation” function related to transcription.[10] This is because a purified human SWI/SNF complex mediated the ATP-dependent disruption of a nucleosomal barrier, resulting in SWI/SNF activators (GAL4-VP16 and GAL 4-AH) binding onto the nucleosome core.[11] Since the TATA sequence is inside a nucleosome, adding ATP will cause human SWI/SNF to recognize its chromatin structure and alter the nucleosomal DNA sequence so that the TPB can access and bind to it.[10] From a broader perspective, this allows for more eukaryotic gene expression, since a variety of eukaryotic promoters will be regulated.[10]
Advancements in biotechnology
editBecause Polycomb repressive complex 1 (PRC1) contains a number of proteins that work together to repress SWI/SNF complex chromatin remodeling, Kingston refined a method to reconstitute a stable complex of proteins that together form a “chromatin structure” that excludes human SWI/SNF.[12] Kingston found that in order to form the complex that silences chromatin remodeling, it must be stable and compact.[13] Through electron microscopy, he found that the components of PRC 1 induce compaction of nucleosomal arrays.[13] The compaction of chromatin occurs within the presence of three nucleosomes and a region of Posterior Sex Combs together.[13] His work with Polycomb proteins further extends, as he helped develop a RIP-sequence method to capture the Polycomb repressive complex 2 (PRC2) transcriptome in embryonic stem cells.[14] Noting that Polycomb proteins factor into stem cell renewal and the formation of diseases, Kingston's discovery of direct interactions (Ezh2 subunit) and PRC2 cofactors (Gtl2 RNA) really contributed to identifying the function of Polycomb proteins within the genome.[14] Dr. Kingston's heavy interest in chromatin remodeling also showed through his research regarding purifying the proteins associated with chromatin remodeling.[15] He established a protocol, Proteomics of Isolated Chromatin Segments (PICh), where a specific nucleic acid probe is used to isolate genomic DNA with regards to the quantity and purity of associated proteins.[15] The PlCh protocol was then used on telomeric chromatin to identify telomeric factors and resulted in finding a number of novel associations.[15] Professor Kingston's advancements within the field of biotechnology extend into developing eukaryotic cell transfection protocols, for he also developed two methods of calcium phosphate transfection for transient and stable transfections.[16] These two methods use a precipitate to introduce plasmid DNA into monolayer cell cultures.[16] The difference between them is that one uses a HEPES-buffered solution while the other uses a BES-buffered system, but both form a precipitate over the cells and allow for similar levels of transient expression.[16]
Macromolecular interaction in chromatin remodeling
editKingston's research surrounding chromatin remodeling dwells into understanding how long non-coding RNAs (lncRNAs) play a role on chromatin binding sites.[17] He was able to genome map NEAT1 and MALAT (both lncRNAs) and found that they localize overactive genes.[17] His research also suggests that NEAT1 and MALAT interact with complementary proteins.[17] He found that underlying DNA sequences are not responsible for targeting NEAT1 to chromatin, but it is rather transcriptional sequences that allow it to bind onto chromatin sites.[17] Robert Kingston's work with lncRNAs extends, as he also discovered that DIGIT interacts with the Bromodomain-containing protein 3 (BRD3).[18] He found that they work together to regulate endoderm differentiation transcriptionally.[18]
Kingston found another breakthrough: that a protein-protein interaction affected chromatin remodeling in the lymphoid system.[19] He discovered that the Ikaros-NURD complex is able to target chromatin remodeling and histone deacetylation complexes in vivo.[19] This allowed him to conclude that chromatin remodeling affects lymphocyte differentiation.[19]
Advances in structural and functional biochemistry
editOne of the biggest discoveries that Robert Kingston found was that the nucleosome structure could be arranged into different conformations so that different biophysical properties can result, including mechanisms of transcription.[20] Specifically, multiprotein complexes that were used for transcriptional regulation were found to acetylate nucleosomes, deacetylate nucleosomes, or alter nucleosome structure when ATP was present.[20] These alterations would essentially be a major way to regulate eukaryotic gene expression.[20] Kingston furthered this and discovered the novel nucleosome remodelling and deacetylating (NRD) complex.[21] Through in vitro studies with CHD3 and CHD4 proteins with ATPase domains found in chromatin remodelling factors, Dr. Kingston established that there was a functional and physical link between nucleosome remodeling proteins and histone deacetylases’ chromatin-modifying features.[21]
Selected review publications
edit- The CBX family of proteins in transcriptional repression and memory
- Cooperation between complexes that regulate chromatin structure and transcription
- Mechanisms of polycomb gene silencing: knowns and unknowns
- Occupying chromatin: Polycomb mechanisms for getting to genomic targets, stopping transcriptional traffic, and staying put
- ATP-dependent remodeling and acetylation as regulators of chromatin fluidity
- Characterization of the piRNA complex from rat testes
- Comparative analysis of metazoan chromatin organization
References
edit- ^ a b c d e f g h "Robert Kingston". www.nasonline.org.
- ^ a b c d "Genetics". genetics.hms.harvard.edu. Retrieved 2021-04-16.
- ^ mghresearch (2023-01-31). "Kingston Ready for New Challenges as Mass General's First Chief Academic Officer". Bench Press. Retrieved 2024-01-28.
- ^ a b Kingston, Robert E.; Chamberlin, Michael J. (1981-12-01). "Pausing and attenuation of in vitro transcription in the rrnB operon of E. coli". Cell. 27 (3): 523–531. doi:10.1016/0092-8674(81)90394-9. ISSN 0092-8674. PMID 6086107. S2CID 19331708.
- ^ Kingston, Robert E.; Baldwin, Albert S.; Sharp, Phillip A. (November 1984). "Regulation of heat shock protein 70 gene expression by c- myc". Nature. 312 (5991): 280–282. doi:10.1038/312280a0. ISSN 1476-4687. PMID 6438521. S2CID 2336314.
- ^ a b Wu, B. J.; Kingston, R. E.; Morimoto, R. I. (1986-02-01). "Human HSP70 promoter contains at least two distinct regulatory domains". Proceedings of the National Academy of Sciences. 83 (3): 629–633. doi:10.1073/pnas.83.3.629. ISSN 0027-8424. PMC 322917. PMID 3456160.
- ^ "Google Scholar". scholar.google.com. Retrieved 2021-04-16.
- ^ Larson, Jeffrey S.; Schuetz, Thomas J.; Kingston, Robert E. (September 1988). "Activation in vitro of sequence-specific DNA binding by a human regulatory factor". Nature. 335 (6188): 372–375. doi:10.1038/335372a0. ISSN 1476-4687. PMID 3419505. S2CID 4336885.
- ^ a b c Kadam, Shilpa; McAlpine, Glenn S.; Phelan, Michael L.; Kingston, Robert E.; Jones, Katherine A.; Emerson, Beverly M. (2000-10-01). "Functional selectivity of recombinant mammalian SWI/SNF subunits". Genes & Development. 14 (19): 2441–2451. doi:10.1101/gad.828000. ISSN 0890-9369. PMC 316972. PMID 11018012.
- ^ a b c Imbalzano, Anthony N.; Kwon, Hyockman; Green, Michael R.; Kingston, Robert E. (August 1994). "Facilitated binding of TATA-binding protein to nucleosomal DNA". Nature. 370 (6489): 481–485. doi:10.1038/370481a0. ISSN 1476-4687. PMID 8047170. S2CID 4337727.
- ^ Kwon, Hyockman; Imbalzano, Anthony N.; Khavari, Paul A.; Kingston, Robert E.; Green, Michael R. (August 1994). "Nucleosome disruption and enhancement of activator binding by a human SW1/SNF complex". Nature. 370 (6489): 477–481. doi:10.1038/370477a0. ISSN 1476-4687. PMID 8047169. S2CID 4337725.
- ^ Francis, Nicole J.; Saurin, Andrew J.; Shao, Zhaohui; Kingston, Robert E. (2001-09-01). "Reconstitution of a Functional Core Polycomb Repressive Complex". Molecular Cell. 8 (3): 545–556. doi:10.1016/S1097-2765(01)00316-1. ISSN 1097-2765. PMID 11583617.
- ^ a b c Francis, Nicole J.; Kingston, Robert E.; Woodcock, Christopher L. (2004-11-26). "Chromatin Compaction by a Polycomb Group Protein Complex". Science. 306 (5701): 1574–1577. doi:10.1126/science.1100576. ISSN 0036-8075. PMID 15567868. S2CID 29551452.
- ^ a b Zhao, Jing; Ohsumi, Toshiro K.; Kung, Johnny T.; Ogawa, Yuya; Grau, Daniel J.; Sarma, Kavitha; Song, Ji Joon; Kingston, Robert E.; Borowsky, Mark; Lee, Jeannie T. (2010-12-22). "Genome-wide Identification of Polycomb-Associated RNAs by RIP-seq". Molecular Cell. 40 (6): 939–953. doi:10.1016/j.molcel.2010.12.011. ISSN 1097-2765. PMC 3021903. PMID 21172659.
- ^ a b c Déjardin, Jérôme; Kingston, Robert E. (2009-01-09). "Purification of Proteins Associated with Specific Genomic Loci". Cell. 136 (1): 175–186. doi:10.1016/j.cell.2008.11.045. ISSN 0092-8674. PMC 3395431. PMID 19135898.
- ^ a b c Kingston, Robert E.; Chen, Claudia A.; Rose, John K. (2003). "Calcium Phosphate Transfection". Current Protocols in Molecular Biology. 63 (1): 9.1.1–9.1.11. doi:10.1002/0471142727.mb0901s63. ISSN 1934-3647. PMID 18265332. S2CID 46188175.
- ^ a b c d West, Jason A.; Davis, Christopher P.; Sunwoo, Hongjae; Simon, Matthew D.; Sadreyev, Ruslan I.; Wang, Peggy I.; Tolstorukov, Michael Y.; Kingston, Robert E. (2014-09-04). "The Long Noncoding RNAs NEAT1 and MALAT1 Bind Active Chromatin Sites". Molecular Cell. 55 (5): 791–802. doi:10.1016/j.molcel.2014.07.012. ISSN 1097-2765. PMC 4428586. PMID 25155612.
- ^ a b Daneshvar, Kaveh; Ardehali, M. Behfar; Klein, Isaac A.; Hsieh, Fu-Kai; Kratkiewicz, Arcadia J.; Mahpour, Amin; Cancelliere, Sabrina O. L.; Zhou, Chan; Cook, Brett M.; Li, Wenyang; Pondick, Joshua V. (October 2020). "lncRNA DIGIT and BRD3 protein form phase-separated condensates to regulate endoderm differentiation". Nature Cell Biology. 22 (10): 1211–1222. doi:10.1038/s41556-020-0572-2. ISSN 1476-4679. PMC 8008247. PMID 32895492.
- ^ a b c Kim, John; Sif, Saïd; Jones, Beverly; Jackson, Audrey; Koipally, Joseph; Heller, Elizabeth; Winandy, Susan; Viel, Alain; Sawyer, Alan; Ikeda, Toru; Kingston, Robert; Georgopoulos, Katia (1999-03-01). "Ikaros DNA-Binding Proteins Direct Formation of Chromatin Remodeling Complexes in Lymphocytes". Immunity. 10 (3): 345–355. doi:10.1016/S1074-7613(00)80034-5. ISSN 1074-7613. PMID 10204490.
- ^ a b c Workman, J. L.; Kingston, R. E. (June 1998). "Alteration of Nucleosome Structure as a Mechanism of Transcriptional Regulation". Annual Review of Biochemistry. 67 (1): 545–579. doi:10.1146/annurev.biochem.67.1.545. ISSN 0066-4154. PMID 9759497.
- ^ a b Tong, Jeffrey K.; Hassig, Christian A.; Schnitzler, Gavin R.; Kingston, Robert E.; Schreiber, Stuart L. (October 1998). "Chromatin deacetylation by an ATP-dependent nucleosome remodelling complex". Nature. 395 (6705): 917–921. doi:10.1038/27699. ISSN 1476-4687. PMID 9804427. S2CID 4355885.