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Query: EC:2.4.2.30 (
PARP
)
13,611
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
This work identifies central components of a feedback mechanism for the expression of mouse poly(ADP-ribose) polymerase-1 (
PARP-1
). Using the stress-induced duplex destabilization algorithm, multiple base-unpairing regions (BURs) could be localized in the 5' region of the mouse
PARP-1
gene (muPARP-1). Some of these could be identified as scaffold/matrix-attachment regions (S/MARs), suggesting an S/
MAR
-mediated transcriptional regulation.
PARP-1
binding to the most proximal element, S/
MAR
1, and to three consensus motifs, AGGCC, in its own promoter (basepairs -956 to +100), could be traced by electrophoretic mobility-shift assay. The AGGCC-complementary GGCCT motif was detected by cis-diammine-dichloro platinum cross-linking and functionally characterized by the effects of site-directed mutagenesis on its performance in wild type (
PARP-1
(+/+)) and
PARP-1
knockout cells (
PARP-1
(-/-)). Mutation of the central AGGCC tract at basepairs -554 to -550 prevented
PARP-1
/promoter interactions, whereby muPARP-1 expression became up-regulated. Transfection of a series of reporter gene constructs with or without S/
MAR
1 (basepairs -1523 to -1007) and the more distant S/
MAR
2 (basepairs -8373 to -6880), into
PARP-1
(+/+) as well as
PARP-1
(-/-) cells, revealed an additional, major level of muPARP-1 promoter down-regulation, triggered by
PARP-1
binding to S/
MAR
1. We conclude that S/
MAR
1 represents an upstream control element that acts in conjunction with the muPARP-1 promoter. These interactions are part of a negative autoregulatory loop.
...
PMID:PARP-1 expression in the mouse is controlled by an autoregulatory loop: PARP-1 binding to an upstream S/MAR element and to a novel recognition motif in its promoter suppresses transcription. 1930 24
Using computer stress-induced duplex destabilization (SIDD) analysis and binding experiments, we identified a S/
MAR
element (-599/-200 bp) (Hp-S/
MAR
) adjacent to the cis-element (-165/-56 bp) in the rat haptoglobin gene. We examined its functional interactions with the lamins and lamin-associated proteins in the basal state and during acute-phase (AP) response-induced increased transcription. Colocalization, electrophoretic mobility shift assay (EMSA), and re-electrophoresis of nucleoprotein complexes, South-Western and Western blot analysis and coimmunoprecipitation experiments revealed that the lamins,
PARP-1
, C/EBP beta, and Hp-S/
MAR
assembled higher order complexes through direct lamin-Hp-S/
MAR
and probably
PARP-1
-Hp-S/
MAR
interactions although C/EBP beta did not bind to the Hp-S/
MAR
but established direct interaction with
PARP-1
. The transition from constitutive to increased haptoglobin gene transcription during the AP response was associated with quantitative and qualitative changes in Hp-S/
MAR
-protein interactions, respectively, observed as increased association of the lamin(s) with the Hp-S/
MAR
and as the appearance of a 90 kDa Hp-S/
MAR
-binding protein. Also, during the AP response the contact between C/EBP beta and
PARP-1
established in the basal state was lost. DNA chromatography with the haptoglobin cis-element and Western blot analysis suggests that
PARP-1
was a coactivator during constitutive and elevated transcription. The results show that the lamin components of the nuclear matrix form a network of functional, dynamic protein-protein and protein-Hp-S/
MAR
associations with multiple partners, and underline the involvement of
PARP-1
in the regulation of haptoglobin gene transcription. We concluded that the interplay of these interactions fine tunes haptoglobin gene expression to meet the changing requirements of liver cells.
...
PMID:Regulation of rat haptoglobin gene expression is coordinated by the nuclear matrix. 1952 70
The poly(adenosine diphosphate (ADP)-ribose) polymerase (
PARP
) protein family generates ADP-ribose (ADPr) modifications onto target proteins using NAD(+) as substrate. Based on the composition of three NAD(+) coordinating amino acids, the H-Y-E motif, each
PARP
is predicted to generate either poly(ADPr) (PAR) or mono(ADPr) (
MAR
). However, the reaction product of each
PARP
has not been clearly defined, and is an important priority since PAR and
MAR
function via distinct mechanisms. Here we show that the majority of PARPs generate
MAR
, not PAR, and demonstrate that the H-Y-E motif is not the sole indicator of
PARP
activity. We identify automodification sites on seven PARPs, and demonstrate that
MAR
and PAR generating PARPs modify similar amino acids, suggesting that the sequence and structural constraints limiting PARPs to
MAR
synthesis do not limit their ability to modify canonical amino-acid targets. In addition, we identify cysteine as a novel amino-acid target for ADP-ribosylation on PARPs.
...
PMID:Family-wide analysis of poly(ADP-ribose) polymerase activity. 2504 79
Protein ADP-ribosylation is a posttranslational modification (PTM) that plays an important role in all major cellular processes, including DNA repair, cellular signaling, and RNA metabolism. Site identification for this PTM has recently become possible through the development of several mass spectrometry-based methods, a critical step in understanding the regulatory role played by mono(ADP-ribose) (
MAR
), poly(ADP-ribose) (PAR), and the enzymes which make these modifications: poly(ADP-ribose) polymerases (PARPs), best known for their role in DNA repair and as targets for chemotherapeutic
PARP
inhibitors. Here, we have described our method for enriching and identifying ADP-ribosylation events through the use of a phosphodiesterase to digest protein-conjugated ADP-ribose down to its attachment structure, phosphoribose. We also include here a guide to choosing between collision-induced dissociation (CID)-, higher-energy collisional dissociation (HCD)-, and electron-transfer dissociation (ETD)-based peptide fragmentation for the identification of phosphoribosylated peptides.
...
PMID:ADP-Ribosylated Peptide Enrichment and Site Identification: The Phosphodiesterase-Based Method. 2869 5
Mono-ADP-ribosylation is a posttranslational modification, which is catalyzed in cells by certain members of the
ADP-ribosyltransferase
diphtheria toxin-like family (ARTD) of ADP-ribosyltransferases (aka
PARP
enzymes). It involves the transfer of a single residue of ADP-ribose (ADPr) from the cofactor NAD
+
onto substrate proteins. Although 12 of the 17 members of the ARTD family have been defined as mono-ARTDs in in vitro assays, relatively little is known about their exact cellular functions. A major challenge is the detection of mono-ADP-ribosylated (MARylated) proteins in cells as no antibodies are available that detect exclusively MARylated proteins. As an alternative to classical antibodies, the
MAR
-specific binding domains macro2 and macro3 of Artd8 can be utilized alone or in combination, to demonstrate intracellular auto-modification levels of ARTD10 in cells in both co-immunoprecipitation and co-localization experiments. Here we demonstrate that different macrodomain constructs of human ARTD8 and murine Artd8, alone or in combination, exert differences with regard to their interaction with ARTD10 in cells. Precisely, while the macrodomains of murine Artd8 interacted with ARTD10 in cells in a MARylation-dependent manner, the macrodomains of human ARTD8 interacted with ARTD10 independent of its catalytic activity. Moreover, we show that a combination of macro2 and macro3 of murine Artd8 was recruited more efficiently to ARTD10 during co-localization experiments compared to the single domains. Therefore, murine Artd8 macrodomain constructs can serve as a tool to evaluate intracellular ARTD10 auto-modification levels using the described methods, while the human ARTD8 macrodomains are less suited because of ADPr-independent binding to ARTD10. Protocols for co-immunoprecipitation and co-localization experiments are described in detail.
...
PMID:Assessment of Intracellular Auto-Modification Levels of ARTD10 Using Mono-ADP-Ribose-Specific Macrodomains 2 and 3 of Murine Artd8. 3009 60
The poly(ADP-ribose) polymerase (
PARP
) family of proteins utilize NAD
+
as the substrate to modify protein acceptors with either mono(ADP-ribose) (
MAR
) or poly(ADP-ribose) (PAR).
MAR
and PAR have been shown to regulate distinct cellular processes. Iso-ADP-ribose (iso-ADPr) is the smallest internal PAR structural unit containing the characteristic ribose-ribose glycosidic bond formed during poly(ADP-ribosyl)ation. The WWE domain of RNF146 specifically recognizes the iso-ADPr moiety in PAR but does not interact with
MAR
. This provides a way to distinguish PAR from
MAR
modification and to isolate PARylated proteins. Iso-ADPr can be used to detect the PAR-specific binding properties of interested proteins. Here we describe the detailed method to generate and purify iso-ADPr and its use in PAR-binding analysis through isothermal titration calorimetry (ITC) analysis.
...
PMID:Biochemical and Biophysical Assays of PAR-WWE Domain Interactions and Production of iso-ADPr for PAR-Binding Analysis. 3009 61
ADP-ribosylation is a covalent posttranslational modification of proteins that is catalyzed by various types of
ADP-ribosyltransferase
(
ART
) enzymes, including members of the poly(ADP-ribose) polymerase (
PARP
) family. ADP-ribose (ADPR) modifications can occur as mono(ADP-ribosyl)ation, oligo(ADP-ribosyl)ation, or poly(ADP-ribosyl)ation, depending on the particular
ART
enzyme catalyzing the reaction, as well as the specific reaction conditions. Understanding the biology of ADP-ribosylation requires facile and robust means of generating and detecting the modification in all of its forms. Here we describe how to generate protein-linked mono(ADP-ribose), oligo(ADP-ribose), and poly(ADP-ribose) (
MAR
, OAR, and PAR, respectively) in vitro as an automodification of PARPs 1 or 3. First, epitope-tagged
PARP-1
(a
PARP
polyenzyme) and PARP-3 (a
PARP
monoenzyme) are expressed individually in insect cells using baculovirus expression vectors, and purified using immunoaffinity chromatography. Second, the purified recombinant PARPs are incubated individually in the presence of different concentrations of NAD
+
(as a donor of ADPR groups) and sheared DNA (to activate their catalytic activities) resulting in various forms of auto-ADP-ribosylation. Third, the products are confirmed using ADPR detection reagents that can distinguish among
MAR
, OAR, and PAR. Finally, if desired, the OAR and PAR can be deproteinized. The protein-linked and free
MAR
, OAR, and PAR generated in these reactions can be used as standards, substrates, or binding partners in a variety of ADPR-related assays.
...
PMID:Generating Protein-Linked and Protein-Free Mono-, Oligo-, and Poly(ADP-Ribose) In Vitro. 3120 27
DNA-dependent poly(ADP-ribose) polymerases (PARPs) PARP1, PARP2 and PARP3 act as DNA break sensors signalling DNA damage. Upon detecting DNA damage, these PARPs use nicotine adenine dinucleotide as a substrate to synthesise a monomer or polymer of ADP-ribose (
MAR
or PAR, respectively) covalently attached to the acceptor residue of target proteins. Recently, it was demonstrated that PARP1-3 proteins can directly ADP-ribosylate DNA breaks by attaching
MAR
and PAR moieties to terminal phosphates. Nevertheless, little is still known about the mechanisms governing substrate recognition and specificity of PARP1, which accounts for most of cellular PARylation activity. Here, we characterised PARP1-mediated DNA PARylation of DNA duplexes containing various types of breaks at different positions. The 3'-terminal phosphate residue at double-strand DNA break ends served as a major acceptor site for PARP1-catalysed PARylation depending on the orientation and distance between DNA strand breaks in a single DNA molecule. A preference for ADP-ribosylation of DNA molecules containing 3'-terminal phosphate over PARP1 auto-ADP-ribosylation was observed, and a model of DNA modification by PARP1 was proposed. Similar results were obtained with purified recombinant PARP1 and HeLa cell-free extracts. Thus, the biological effects of
PARP
-mediated ADP-ribosylation may strongly depend on the configuration of complex DNA strand breaks.
...
PMID:Insight into DNA substrate specificity of PARP1-catalysed DNA poly(ADP-ribosyl)ation. 3211 79
