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Lecture_Chromatin remodelling_slideshare.pdf

Kristu Jayanti College
Kristu Jayanti College

1. Chromatin remodeling complexes use ATP hydrolysis to modify nucleosome structure and expose DNA for gene expression. The main classes are ATP-independent complexes and ATP-dependent complexes like ISWI and SWI/SNF. 2. Post-translational modifications of histone tails like acetylation, methylation, and phosphorylation can affect chromatin structure and transcription by altering DNA-histone interactions. 3. Chromatin remodeling is important for differential gene expression in specialized cell types and controlling DNA accessibility for transcription.

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K. Narayanapura, Kothanur (PO), Bengaluru 560077 www.kristujayanti.edu.in Chromatin Remodelling Dr. Manikandan Kathirvel Assistant Professor, Department of Life Sciences, Kristu Jayanti College (Autonomous), Bengaluru
Chromatin Remodeling • Chromatin structure provides an important level of control of gene transcription. • The development of specialized organs, tissues, and cells and their function in the intact organism depend upon the differential expression of genes. • Some of this differential expression is achieved by having different regions of chromatin available for transcription in cells from various tissues. Large regions of chromatin are transcriptionally inactive in some cells, while they are either active or potentially active in other specialized cells. For example, the DNA containing the - globin gene cluster is in "active" chromatin in the reticulocytes but in "inactive" chromatini n muscle cells.
MAJOR CLASSES OF CHROMATIN-REMODELING COMPLEXES Chromatin remodeling complex ATP Independent modeling complexes ATP Dependent modeling complexes Histone modifications The ATP dependent remodeling complexes require ATP hydrolysis for modification of architecture of nucleosome which helps to expose the required sequence in DNA for gene expression. The enzymes are as follows: ISWI (imitation switch ) SWI/SNF (Switching of mating types/ sucrose non fermenting)
EFFECTS OF HISTONES ON TRANSCRIPTION ACTIVATION  Histone modification – post translational modification includes methylation, phosphorylation, acetylation, ubiquitylation, summoylation.  DNA wrap around the histone octamer in a structure like beads on string ,which makes the basic chromatin unit.  Chromatin folds into higher level structures, helps to determine the DNA accessibility.  The transcriptional machinery cannot access the DNA and genes remain inactive.
Histones  Histones are a group of basic proteins that associate with DNA to condense it into chromatin.  Histones contain a large proportion of the positively charged (basic) amino acids , lysine and arginine in their structure.  DNA is negatively charged due to the phosphate groups on its backbone.  The results of these attraction and therefore high binding affinity between histones and DNA structure called nucleosomes.  DNA wraps around histones, they also play a role in gene regulation.  The basic unit of chromatin is the nucleosome core particles, which contains 147 bp of DNA wrapped nearly twice around an octamer of the core histones.  Each nucleosome is separated by 10-60 bp of “linker” DNA, and the resulting nucleosomal array constitutes a chromatin fiber of 10 nm in diameter.
 Two types of Histones: 1) Core Histones- H2A, H2B, H3, H4 2) Linker Histones- H1  The eight histones in the core are arranged into a (H3)2(H4)2 tetramer and a pair of H2A-H2B dimers.  The tetramer and dimers come together to form a left- handed superhelical ramp around which the DNA wraps.  Hydrogen bonds between the DNA backbone and the amide group on the main chain of histone proteins.
Formation and disruption of nucleosome structure: • The presence of nucleosomes and of complexes of histones and DNA provide a barrier against the ready association of transcription factors with specific DNA regions. 1. Chromatin composed of cells DNA and associated proteins. 2. There are five histone proteins in the family H1,H2A,H2B,H3,and H4. 3. Two H3 and two H4 proteins form a tetramer which combines with two H2A,H2B dimers to form the disk shaped histone core . 4. 150bp of DNA wrap around the protein about twice making a nucleosome core particle with linker histone and linker DNA. 5. Linker DNA varies in length ( 10 and 90bp). 6. Nucleosome repeats every 200bp and is close to 10nm diameter.
Histone modification  N-terminal tails of histones are the most accessible regions of these peptides as they protrude from the nucleosome and possess no specific structure. The amino-terminal portion of the core histone proteins contains a flexible and highly basic tail region, which is conserved across various species and is subject to various PTM. Chromatin can be highly packed or loosely packed, and correlated to the gene expression levels. Post-translational modifications(PTM) of histones is a crucial step in epigenetic regulation of a gene. Modifications in histone proteins affects the structure of chromatin. Gene regulation DNA damage and repair Chromosome condensation
Types of histone modification  N-terminal tails of all histones are particularly of interest since they protrude out of the compact structure. These N-terminal tails are often subjected to a variety of post-translational modifications such as, a) Acetylation b) Methylation c) Phosphorylation d) Ubiquitination e) Sumoylation f) ADP ribosylation
The disruption of nucleosome structure is therefore an important part of eukaryotic gene regulation and the processes involved are as follows: i) Histone acetylation and deacetylation Acetylation is known to occur on lysine residues in the amino terminal tails of histone molecules. This modification reduces the positive charge of these tails and decreases the binding affinity of histone for the negatively charged DNA. Accordingly, the acetylation of histones could result in disruption of nucleosomal structure and allow readier access of transcription factors to cognate regulatory DNA elements.
N-terminal tails are reversible acetylated in Lys, particularly in H3+H4.  Acetyl group addition to lysine in histone tails loosens nucleosome grip on DNA by neutralizing positive charge. i) Histone acetylation and deacetylation
i) Histone acetylation and deacetylation
ATP INDEPENDENT REMODELING COMPLEX
ii) Methylation  It is the introduction of an methyl functional group to only on Lysine or Arginine of the histone tail.  These reactions are catalysed by enzymes like histone methyltransferases (HMTs).  Histone lysine methyl transferases (HKMTs) methylate Lysine (K) residues.  Protein argenine methyl transferases (PRMTs) methylate Arginine (R) residues.  A role in both activation and repression.  Arginines can be mono or di methylated whereas lysines can be mono, di , tri methylated.
ii) Methylation Methylation of deoxycytidine residues in DNA may effect gross changes in chromatin so as to preclude its active transcription. Example: Acute demethylation of deoxycytidine residues in a specific region of the tyrosine aminotransferase gene—in response to glucocorticoid hormones—has been associated with an increased rate of transcription of the gene.
iii) Ubiquitination  Ubiquitination (or ubiquitylation) refers to the post translational modification of the amino group of a lysine residue by the covalent attachment of one (monoubiquitination) or more (polyubiquitination) ubiquitin monomers.  Ubiquitin is a 76 amino acid protein highly conserved in eukaryotes.  Histone Ubiquitination alters chromatin structure and allows the access of enzymes involved in transcription.  Ubiquitination is carried out in three steps: activation, conjugation and ligation, performed by ubiquitin- activating enzymes (E1s), ubiquitin- conjugating enzymes (E2s) and ubiquitin ligases (E3s), respectively.
v) Sumoylation:  Small ubiquitin like modifier (SUMO) proteins are a family of small proteins that are attached to and detached from other proteins in cell to modify their function.  Sumoylation consists in the addition of a small ubiquitin related modifier protein (SUMO) of 100 amino acids.  Histone Sumoylation has a role in transcription repression by opposing other active marks such as Acetylation, methylation, Ubiquitination, etc. iv) Phosphorylation  Phosphorylation is the addition of a phosphate group (PO43-) to a molecule.  Phosphorylation is catalyzed by various specific protein kinases.  Histones are phosphorylated and the most studied sites of histone Phosphorylation are the serine 10 of histone H3 (H3S10)
vi) DNA binding proteins •The binding of specific transcription factors to certain DNA elements may result in disruption of nucleosomal structure. •Many eukaryotic genes have multiple protein-binding DNA elements. •The serial binding of transcription factors to these elements may either directly disrupt the structure of the nucleosome or prevent its re-formation. •These reactions result in chromatin-level structural changes that in the end increase DNA accessibility to other factors and the transcription machinery.
Studies postulate that SWI2/SNF2 and related proteins can function to destabilize nucleosome structure and thereby to facilitate the binding of transcription factors to chromatin. SWI2/SNF2: Genetic studies of transcriptional regulation in Saccharomyces cerevisiae led to the identification of a number of SWI and SNF genes (SWI refers to yeast mating type swi tching, while SNF is an abbreviation for s ucrose n on f ermenting. The gene encoding the first SNF2/SWI2 enzyme was discovered by the yeast geneticists Ira Herskowitz and Marian Carlson in the 1980s.
SNF2 protein A SNF2 protein is an enzyme that belongs to the SF2 helicase- like superfamily, and it is the founding member of a subfamily of enzymes called SNF2-like helicases, which all harbor a conserved helicase-related motifs similar to SNF2. The SNF2 family proteins have multiple members, which are approximately 30 different enzymes in human cells and 17 different enzymes in budding yeast. SNF2 enzymes can be further classified into six groups based on the structure of the helicase domain. These groups are Swi2/Snf2-like, Swr1-like, SS01653-like, Rad54-like, Rad5/6- like, and distant (SMARCAL1) enzymes.  Many of the SNF2 enzymes have been shown to remodel chromatin in vitro in an ATP-dependent manner, and several enzymes remain to be tested.
SWI2/SNF2 Complex: Experiments revealed that the SWI/SNF complex possesses a DNA- stimulated ATPase activity and can destabilize histone-DNA interactions in reconstituted nucleosomes in an ATP-dependent manner, though the exact nature of this structural change is not known. In addition, this SWI2/SNF2-mediated destabilization of nucleosomes was found to increase the binding of transcription factors, such as GAL4 derivatives or the TATA box-binding protein (TBP), to the histone-associated DNA. These results, combined with the genetic data, led to the hypothesis that the SWI/SNF complex facilitates the binding of transcription factors to chromatin.
A Simple Model Depicting a Suggested Mechanism for the Destabilization of Nucleosomes by SWI/SNF Complex and Related Factors by ATP-Driven Translocation of the Protein along Nucleosomal DNA ATP DEPENDENT REMODELING COMPLEXES
Members of the SNF2-like family exhibit an impressive range of biological functions. These activities include •gene-specific transcriptional activation, •transcriptional repression, •destabilization of reconstituted nucleosomes, •transcription-coupled repair, •nucleotide excision repair of nontranscribed regions of the genome, •recombination repair, •and chromosome segregation. SNF2-like family members are also involved in human disease. •Mutations in the human ERCC6 gene can lead to Cockayne's syndrome, which is characterized by progressive neurodegeneration, dwarfism, photosensitivity, and developmental abnormalities. • In addition, mutated forms of the human ATR-X gene (also known as NUCPRO; tentatively assigned to the RAD54 subfamily) cause a combined α-thalassemia and mental retardation syndrome
NURF—A Complex Containing ISWI, a Member of the SNF2L Subfamily The analysis of an ATP-dependent activity that is required to alter nucleosome structure upon binding of the GAGA transcription factor (a sequence-specific DNA-binding factor in Drosophila) has led to the purification of a factor termed NURF (Nucleosome Remodeling Factor) from Drosophila embryos. NURF is an ∼0.5 MDa complex that contains four polypeptides, one of which is the ISWI (imitation switch) protein. ISWI is a member of the SNF2L subfamily, which is closely related to the SNF2 subfamily. At present, downstream targets of ISWI are not known. ISWI, a Member of the SWI2/SNF2 ATPase Family, Encodes the 140 kDa Subunit of the Nucleosome Remodeling Factor

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Lecture_Chromatin remodelling_slideshare.pdf

  • 1. K. Narayanapura, Kothanur (PO), Bengaluru 560077 www.kristujayanti.edu.in Chromatin Remodelling Dr. Manikandan Kathirvel Assistant Professor, Department of Life Sciences, Kristu Jayanti College (Autonomous), Bengaluru
  • 2. Chromatin Remodeling • Chromatin structure provides an important level of control of gene transcription. • The development of specialized organs, tissues, and cells and their function in the intact organism depend upon the differential expression of genes. • Some of this differential expression is achieved by having different regions of chromatin available for transcription in cells from various tissues. Large regions of chromatin are transcriptionally inactive in some cells, while they are either active or potentially active in other specialized cells. For example, the DNA containing the - globin gene cluster is in "active" chromatin in the reticulocytes but in "inactive" chromatini n muscle cells.
  • 3. MAJOR CLASSES OF CHROMATIN-REMODELING COMPLEXES Chromatin remodeling complex ATP Independent modeling complexes ATP Dependent modeling complexes Histone modifications The ATP dependent remodeling complexes require ATP hydrolysis for modification of architecture of nucleosome which helps to expose the required sequence in DNA for gene expression. The enzymes are as follows: ISWI (imitation switch ) SWI/SNF (Switching of mating types/ sucrose non fermenting)
  • 4. EFFECTS OF HISTONES ON TRANSCRIPTION ACTIVATION  Histone modification – post translational modification includes methylation, phosphorylation, acetylation, ubiquitylation, summoylation.  DNA wrap around the histone octamer in a structure like beads on string ,which makes the basic chromatin unit.  Chromatin folds into higher level structures, helps to determine the DNA accessibility.  The transcriptional machinery cannot access the DNA and genes remain inactive.
  • 5. Histones  Histones are a group of basic proteins that associate with DNA to condense it into chromatin.  Histones contain a large proportion of the positively charged (basic) amino acids , lysine and arginine in their structure.  DNA is negatively charged due to the phosphate groups on its backbone.  The results of these attraction and therefore high binding affinity between histones and DNA structure called nucleosomes.  DNA wraps around histones, they also play a role in gene regulation.  The basic unit of chromatin is the nucleosome core particles, which contains 147 bp of DNA wrapped nearly twice around an octamer of the core histones.  Each nucleosome is separated by 10-60 bp of “linker” DNA, and the resulting nucleosomal array constitutes a chromatin fiber of 10 nm in diameter.
  • 6.  Two types of Histones: 1) Core Histones- H2A, H2B, H3, H4 2) Linker Histones- H1  The eight histones in the core are arranged into a (H3)2(H4)2 tetramer and a pair of H2A-H2B dimers.  The tetramer and dimers come together to form a left- handed superhelical ramp around which the DNA wraps.  Hydrogen bonds between the DNA backbone and the amide group on the main chain of histone proteins.
  • 7. Formation and disruption of nucleosome structure: • The presence of nucleosomes and of complexes of histones and DNA provide a barrier against the ready association of transcription factors with specific DNA regions. 1. Chromatin composed of cells DNA and associated proteins. 2. There are five histone proteins in the family H1,H2A,H2B,H3,and H4. 3. Two H3 and two H4 proteins form a tetramer which combines with two H2A,H2B dimers to form the disk shaped histone core . 4. 150bp of DNA wrap around the protein about twice making a nucleosome core particle with linker histone and linker DNA. 5. Linker DNA varies in length ( 10 and 90bp). 6. Nucleosome repeats every 200bp and is close to 10nm diameter.
  • 8. Histone modification  N-terminal tails of histones are the most accessible regions of these peptides as they protrude from the nucleosome and possess no specific structure. The amino-terminal portion of the core histone proteins contains a flexible and highly basic tail region, which is conserved across various species and is subject to various PTM. Chromatin can be highly packed or loosely packed, and correlated to the gene expression levels. Post-translational modifications(PTM) of histones is a crucial step in epigenetic regulation of a gene. Modifications in histone proteins affects the structure of chromatin. Gene regulation DNA damage and repair Chromosome condensation
  • 9. Types of histone modification  N-terminal tails of all histones are particularly of interest since they protrude out of the compact structure. These N-terminal tails are often subjected to a variety of post-translational modifications such as, a) Acetylation b) Methylation c) Phosphorylation d) Ubiquitination e) Sumoylation f) ADP ribosylation
  • 10. The disruption of nucleosome structure is therefore an important part of eukaryotic gene regulation and the processes involved are as follows: i) Histone acetylation and deacetylation Acetylation is known to occur on lysine residues in the amino terminal tails of histone molecules. This modification reduces the positive charge of these tails and decreases the binding affinity of histone for the negatively charged DNA. Accordingly, the acetylation of histones could result in disruption of nucleosomal structure and allow readier access of transcription factors to cognate regulatory DNA elements.
  • 11. N-terminal tails are reversible acetylated in Lys, particularly in H3+H4.  Acetyl group addition to lysine in histone tails loosens nucleosome grip on DNA by neutralizing positive charge. i) Histone acetylation and deacetylation
  • 12. i) Histone acetylation and deacetylation
  • 14. ii) Methylation  It is the introduction of an methyl functional group to only on Lysine or Arginine of the histone tail.  These reactions are catalysed by enzymes like histone methyltransferases (HMTs).  Histone lysine methyl transferases (HKMTs) methylate Lysine (K) residues.  Protein argenine methyl transferases (PRMTs) methylate Arginine (R) residues.  A role in both activation and repression.  Arginines can be mono or di methylated whereas lysines can be mono, di , tri methylated.
  • 15. ii) Methylation Methylation of deoxycytidine residues in DNA may effect gross changes in chromatin so as to preclude its active transcription. Example: Acute demethylation of deoxycytidine residues in a specific region of the tyrosine aminotransferase gene—in response to glucocorticoid hormones—has been associated with an increased rate of transcription of the gene.
  • 16.
  • 17. iii) Ubiquitination  Ubiquitination (or ubiquitylation) refers to the post translational modification of the amino group of a lysine residue by the covalent attachment of one (monoubiquitination) or more (polyubiquitination) ubiquitin monomers.  Ubiquitin is a 76 amino acid protein highly conserved in eukaryotes.  Histone Ubiquitination alters chromatin structure and allows the access of enzymes involved in transcription.  Ubiquitination is carried out in three steps: activation, conjugation and ligation, performed by ubiquitin- activating enzymes (E1s), ubiquitin- conjugating enzymes (E2s) and ubiquitin ligases (E3s), respectively.
  • 18. v) Sumoylation:  Small ubiquitin like modifier (SUMO) proteins are a family of small proteins that are attached to and detached from other proteins in cell to modify their function.  Sumoylation consists in the addition of a small ubiquitin related modifier protein (SUMO) of 100 amino acids.  Histone Sumoylation has a role in transcription repression by opposing other active marks such as Acetylation, methylation, Ubiquitination, etc. iv) Phosphorylation  Phosphorylation is the addition of a phosphate group (PO43-) to a molecule.  Phosphorylation is catalyzed by various specific protein kinases.  Histones are phosphorylated and the most studied sites of histone Phosphorylation are the serine 10 of histone H3 (H3S10)
  • 19. vi) DNA binding proteins •The binding of specific transcription factors to certain DNA elements may result in disruption of nucleosomal structure. •Many eukaryotic genes have multiple protein-binding DNA elements. •The serial binding of transcription factors to these elements may either directly disrupt the structure of the nucleosome or prevent its re-formation. •These reactions result in chromatin-level structural changes that in the end increase DNA accessibility to other factors and the transcription machinery.
  • 20. Studies postulate that SWI2/SNF2 and related proteins can function to destabilize nucleosome structure and thereby to facilitate the binding of transcription factors to chromatin. SWI2/SNF2: Genetic studies of transcriptional regulation in Saccharomyces cerevisiae led to the identification of a number of SWI and SNF genes (SWI refers to yeast mating type swi tching, while SNF is an abbreviation for s ucrose n on f ermenting. The gene encoding the first SNF2/SWI2 enzyme was discovered by the yeast geneticists Ira Herskowitz and Marian Carlson in the 1980s.
  • 21. SNF2 protein A SNF2 protein is an enzyme that belongs to the SF2 helicase- like superfamily, and it is the founding member of a subfamily of enzymes called SNF2-like helicases, which all harbor a conserved helicase-related motifs similar to SNF2. The SNF2 family proteins have multiple members, which are approximately 30 different enzymes in human cells and 17 different enzymes in budding yeast. SNF2 enzymes can be further classified into six groups based on the structure of the helicase domain. These groups are Swi2/Snf2-like, Swr1-like, SS01653-like, Rad54-like, Rad5/6- like, and distant (SMARCAL1) enzymes.  Many of the SNF2 enzymes have been shown to remodel chromatin in vitro in an ATP-dependent manner, and several enzymes remain to be tested.
  • 22. SWI2/SNF2 Complex: Experiments revealed that the SWI/SNF complex possesses a DNA- stimulated ATPase activity and can destabilize histone-DNA interactions in reconstituted nucleosomes in an ATP-dependent manner, though the exact nature of this structural change is not known. In addition, this SWI2/SNF2-mediated destabilization of nucleosomes was found to increase the binding of transcription factors, such as GAL4 derivatives or the TATA box-binding protein (TBP), to the histone-associated DNA. These results, combined with the genetic data, led to the hypothesis that the SWI/SNF complex facilitates the binding of transcription factors to chromatin.
  • 23.
  • 24. A Simple Model Depicting a Suggested Mechanism for the Destabilization of Nucleosomes by SWI/SNF Complex and Related Factors by ATP-Driven Translocation of the Protein along Nucleosomal DNA ATP DEPENDENT REMODELING COMPLEXES
  • 25. Members of the SNF2-like family exhibit an impressive range of biological functions. These activities include •gene-specific transcriptional activation, •transcriptional repression, •destabilization of reconstituted nucleosomes, •transcription-coupled repair, •nucleotide excision repair of nontranscribed regions of the genome, •recombination repair, •and chromosome segregation. SNF2-like family members are also involved in human disease. •Mutations in the human ERCC6 gene can lead to Cockayne's syndrome, which is characterized by progressive neurodegeneration, dwarfism, photosensitivity, and developmental abnormalities. • In addition, mutated forms of the human ATR-X gene (also known as NUCPRO; tentatively assigned to the RAD54 subfamily) cause a combined α-thalassemia and mental retardation syndrome
  • 26. NURF—A Complex Containing ISWI, a Member of the SNF2L Subfamily The analysis of an ATP-dependent activity that is required to alter nucleosome structure upon binding of the GAGA transcription factor (a sequence-specific DNA-binding factor in Drosophila) has led to the purification of a factor termed NURF (Nucleosome Remodeling Factor) from Drosophila embryos. NURF is an ∼0.5 MDa complex that contains four polypeptides, one of which is the ISWI (imitation switch) protein. ISWI is a member of the SNF2L subfamily, which is closely related to the SNF2 subfamily. At present, downstream targets of ISWI are not known. ISWI, a Member of the SWI2/SNF2 ATPase Family, Encodes the 140 kDa Subunit of the Nucleosome Remodeling Factor