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Query: UMLS:C0019693 (
HIV
)
170,526
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
We studied human immunodeficiency virus, type 1 (HIV-1) integrase (IN) complexes derived from nuclei of human cells stably expressing the viral protein from a synthetic gene. We show that in the nuclear extracts IN exists as part of a large distinct complex with an apparent Stokes radius of 61 A, which dissociates upon dilution yielding a core molecule of 41 A. We isolated the IN complexes from cells expressing FLAG-tagged IN and demonstrated that the 41 A core is a tetramer of IN, whereas 61 A molecules are composed of IN tetramers associated with a cellular protein with an apparent molecular mass of 76 kDa. This novel integrase interacting protein was found to be identical to lens epithelium-derived growth factor (LEDGF/
p75
), a protein implicated in regulation of gene expression and cellular stress response.
HIV
-1 IN and LEDGF co-localized in the nuclei of human cells stably expressing IN. Furthermore, recombinant LEDGF robustly enhanced strand transfer activity of
HIV
-1 IN in vitro. Our findings indicate that the minimal IN molecule in human cells is a homotetramer, suggesting that at least an octamer of IN is required to accomplish coordinated integration of both retroviral long terminal repeats and that LEDGF is a cellular factor involved in this process.
...
PMID:HIV-1 integrase forms stable tetramers and associates with LEDGF/p75 protein in human cells. 1240 1
We have reported that human immunodeficiency virus type 1 (HIV-1) integrase (IN) forms a specific nuclear complex with human lens epithelium-derived growth factor/transcription co-activator
p75
(LEDGF/
p75
) protein. We now studied the IN-LEDGF/
p75
interaction and nuclear import of IN in living cells using fusions of IN and LEDGF/
p75
with enhanced green fluorescent protein and far-red fluorescent protein HcRed1. We show that both the N-terminal zinc binding domain and the central core domains of IN are involved in the interaction with LEDGF/
p75
. Both domains are essential for nuclear localization of IN as well as for the association of IN with condensed chromosomes during mitosis. However, upon overexpression of LEDGF/
p75
, the core domain fragment of IN was recruited to the nuclei and mitotic chromosomes with a distribution pattern characteristic of the full-length protein, indicating that it harbors the main determinant for interaction with LEDGF/
p75
. Although the C-terminal domain of IN was dispensable for nuclear/chromosomal localization, a fusion of the C-terminal IN fragment with enhanced green fluorescent protein was found exclusively in the nucleus, with a diffuse nuclear/nucleolar distribution, suggesting that the C-terminal domain may also play a role in the nuclear import of IN. In contrast to LEDGF/
p75
, its alternative splice variant, p52, did not interact with
HIV
-1 IN in vitro and in living cells. Finally, RNA interference-mediated knock-down of endogenous LEDGF/
p75
expression abolished nuclear/chromosomal localization of IN. We conclude, therefore, that the interaction with LEDGF/
p75
accounts for the karyophilic properties and chromosomal targeting of
HIV
-1 IN.
...
PMID:LEDGF/p75 is essential for nuclear and chromosomal targeting of HIV-1 integrase in human cells. 1279 94
Human lens epithelium-derived growth factor (LEDGF)/
p75
protein forms a specific nuclear complex with human immunodeficiency virus type 1 (HIV-1) integrase and is essential for nuclear localization and chromosomal association of the viral protein. We now studied nuclear import of LEDGF/
p75
in live and semipermeabilized cells. We show that nuclear import of LEDGF/
p75
is GTP-, Ran-, importin-alpha/beta-, and energy-dependent and that the protein competes with the canonical SV40 large T antigen nuclear localization signal (NLS) for nuclear import receptors. We identified the NLS of LEDGF/
p75
through deletion analysis and site-directed mutagenesis. The LEDGF/
p75
NLS, 148GRKRKAEKQ156, belongs to the canonical SV40-like family. Fusion of this short peptide to the amino terminus of Escherichia coli beta-galactosidase rendered the fusion protein nuclear, confirming that the LEDGF/
p75
NLS is transferable. Moreover, a single amino acid change in the NLS was sufficient to exclude the mutant LEDGF/
p75
protein from the nucleus and abolish nuclear import of
HIV
-1 integrase.
...
PMID:Identification and characterization of a functional nuclear localization signal in the HIV-1 integrase interactor LEDGF/p75. 1516 64
Human immunodeficiency virus type 1 (HIV-1), feline immunodeficiency virus (FIV), and Moloney murine leukemia virus (MoMLV) integrases were stably expressed to determine their intracellular trafficking. Each lentiviral integrase localized to cell nuclei in close association with chromatin while the murine oncoretroviral integrase was cytoplasmic. Fusions of pyruvate kinase to the lentiviral integrases did not reveal transferable nuclear localization signals. The intracellular trafficking of each was determined instead by the transcriptional coactivator LEDGF/
p75
, which was required for nuclear localization. Stable small interfering RNA expression eliminated detectable LEDGF/
p75
expression and caused dramatic, stable redistribution of each lentiviral integrase from nucleus to cytoplasm while the distribution of MoMLV integrase was unaffected. In addition, endogenous LEDGF/
p75
coimmunoprecipitated specifically with each lentiviral integrase. In vitro integration assays with preintegration complexes (PICs) showed that endogenous LEDGF/
p75
is a component of functional
HIV
-1 and FIV PICs. However,
HIV
-1 and FIV infection and replication in LEDGF/
p75
-deficient cells was equivalent to that in control cells, whether cells were dividing or growth arrested. Two-long terminal repeat circle accumulation in nondividing cell nuclei was also equivalent to that of LEDGF/
p75
wild-type cells. Virions produced in LEDGF/
p75
-deficient cells had normal infectivity. We conclude that LEDGF/
p75
fully accounts for cellular trafficking of diverse lentiviral, but not oncoretroviral, integrases and is the main lentiviral integrase-to-chromatin tethering factor. While lentiviral PIC nuclear import is unaffected by LEDGF/
p75
knockdown, this protein is a component of functional lentiviral PICs. A role in
HIV
-1 integration site distribution merits investigation.
...
PMID:LEDGF/p75 determines cellular trafficking of diverse lentiviral but not murine oncoretroviral integrase proteins and is a component of functional lentiviral preintegration complexes. 1530 44
Human lens epithelium-derived growth factor/transcriptional co-activator
p75
(LEDGF/
p75
) protein was recently identified as a binding partner for
HIV
-1 integrase (IN) in human cells. In this work, we used biochemical and bioinformatic approaches to define the domain organization of LEDGF/
p75
. Using limited proteolysis and deletion mutagenesis we show that the protein contains a pair of evolutionarily conserved domains, assuming about 35% of its sequence. Whereas the N-terminal PWWP domain had been recognized previously, the second domain is novel. It is comprised of approximately 80 amino acid residues and is both necessary and sufficient for binding to
HIV
-1 IN. Strikingly, the integrase binding domain (IBD) is not unique to LEDGF/
p75
, as a second human protein, hepatoma-derived growth factor-related protein 2 (HRP2), contains a homologous sequence. LEDGF/
p75
and HRP2 IBDs avidly bound
HIV
-1 IN in an in vitro GST pull-down assay and each full-length protein potently stimulated
HIV
-1 IN activity in vitro. LEDGF/
p75
and HRP2 are predicted to share a similar domain organization and have an evident evolutionary and likely functional relationship.
...
PMID:Identification of an evolutionarily conserved domain in human lens epithelium-derived growth factor/transcriptional co-activator p75 (LEDGF/p75) that binds HIV-1 integrase. 1537 38
The transcriptional coactivator lens epithelium-derived growth factor (LEDGF)/
p75
acts as a chromatin tethering factor for human immunodeficiency virus type 1 (HIV-1) integrase protein, determining its nuclear localization and its tight association with nuclear DNA. Here we identify a second function for the LEDGF/
p75
-integrase interaction. We observed that stable introduction of
HIV
-1 integrase (IN) transcription units into cells made stringently LEDGF/
p75
-deficient by RNAi resulted in much lower steady state levels of IN protein than introduction into LEDGF/
p75
wild type cells. The same LEDGF/
p75
-dependent disparity was observed for feline immunodeficiency virus IN. However, IN mRNA levels were equivalent in the presence and absence of LEDGF/
p75
. A post-translational mechanism was confirmed when the half-life of
HIV
-1 IN protein was found to be much shorter in LEDGF/
p75
-deficient cells. Proteasome inhibition fully countered this extreme instability, increasing IN protein levels to those seen in LEDGF/
p75
wild type cells and implicating proteasomal destruction as the main cause of IN instability. Consistent with these data, increased ubiquitinated
HIV
-1 IN was found in the LEDGF/
p75
knock-down cells. Moreover, restoration of LEDGF/
p75
to knocked down clones rescued
HIV
-1 IN stability. Subcellular fractionation showed that
HIV
-1 IN is exclusively cytoplasmic in LEDGF/
p75
-deficient cells, but mainly nuclear in LEDGF/
p75
wild type cells, and that cytoplasmic
HIV
-1 IN has a shorter half-life than nuclear
HIV
-1 IN. However, using LEDGF proteins defective for nuclear localization and IN interaction, we further determined that protection of
HIV
-1 IN from the proteasome requires neither chromatin tethering nor nuclear residence. Protection requires only interaction with LEDGF/
p75
, and it is independent of the subcellular localization of the IN-LEDGF complex.
...
PMID:Lens epithelium-derived growth factor/p75 prevents proteasomal degradation of HIV-1 integrase. 1547 59
Recently we described the interaction of human immunodeficiency virus type 1 (HIV-1)1 integrase (IN) with a cellular protein, lens epithelium-derived growth factor/transcription co-activator
p75
(LEDGF/
p75
). We now present the study of the diffusion behavior of the three independent domains of IN and LEDGF/
p75
using fluorescence correlation microscopy (FCM). We show that diffusion in the cell of the different enhanced green fluorescent protein (EGFP) fusion proteins is described by two components with different fractions and that the average parameters in the nucleus are comparable with those in the cytoplasm. In addition, we demonstrate that specific interaction between EGFP-fused
HIV
-1 IN and LEDGF/
p75
results in a shift in diffusion coefficient (D). The opposite shift was observed in an IN-deletion mutant that does not exhibit LEDGF/
p75
binding or in a LEDGF/
p75
knock-down experiment using siRNA. We thus demonstrate that protein-protein interactions can be studied in living cells, using single-color FCM (scFCM).
...
PMID:Measuring protein-protein interactions inside living cells using single color fluorescence correlation spectroscopy. Application to human immunodeficiency virus type 1 integrase and LEDGF/p75. 1578 49
To investigate the basis for the LEDGF/
p75
dependence of
HIV
-1 integrase (IN) nuclear localization and chromatin association, we used cell lines made stably deficient in endogenous LEDGF/
p75
by RNAi to analyze determinants of its location in cells and its ability to interact with IN. Deletion of C-terminal LEDGF/
p75
residues 340-417 preserved nuclear and chromatin localization but abolished the interaction with IN and the tethering of IN to chromatin. Transfer of this IN-binding domain (IBD) was sufficient to confer
HIV
-1 IN interaction to GFP. HRP-2, the only other human protein with an identifiable IBD domain, was found to translocate IN to the nucleus of LEDGF/
p75
(-) cells. However, in contrast to LEDGF/
p75
, HRP-2 is not chromatin bound and does not tether IN to chromatin. A single classical nuclear localization signal (NLS) in the LEDGF/
p75
N-terminal region ((146)RRGRKRKAEKQ(156)) was found by deletion mapping and was shown to be transferable to pyruvate kinase. Four central basic residues in the NLS are critical for its activity. Strikingly, however, stable expression studies with NLS(+/-) and IBD(+/-) mutants revealed that the NLS, although responsible for LEDGF/
p75
nuclear import, is dispensable for stable, constitutive nuclear association of LEDGF/
p75
and IN. Both wild-type LEDGF/
p75
and NLS-mutant LEDGF/
p75
remain entirely chromatin associated throughout the cell cycle, and each tethers IN to chromatin. Thus, these experiments reveal stable nuclear sequestration of a transcriptional regulator by chromatin during the nuclear-cytosolic mixing of cell division, which additionally enables stable tethering of IN to chromatin. LEDGF/
p75
is a multidomain adaptor protein that interacts with the nuclear import apparatus, lentiviral IN proteins and chromatin by means of an NLS, an IBD and additional chromatin-interacting domains.
...
PMID:Identification of the LEDGF/p75 HIV-1 integrase-interaction domain and NLS reveals NLS-independent chromatin tethering. 1579 27
The insertion of a DNA copy of its RNA genome into a chromosome of the host cell is mediated by the viral integrase with the help of mostly uncharacterized cellular cofactors. We have recently described that the transcriptional co-activator LEDGF/
p75
strongly interacts with
HIV
-1 integrase. Here we show that interaction of
HIV
-1 integrase with LEDGF/
p75
is important for viral replication. Using multiple approaches including two-hybrid interaction studies, random and directed mutagenesis, we could demonstrate that
HIV
-1 virus harboring a single mutation that disrupts integrase-LEDGF/
p75
interaction, resulted in defective
HIV
-1 replication. Furthermore, we found that LEDGF/
p75
tethers
HIV
-1 integrase to chromosomes and that this interaction may be important for the integration process and the replication of
HIV
-1.
...
PMID:Integrase mutants defective for interaction with LEDGF/p75 are impaired in chromosome tethering and HIV-1 replication. 1585 67
Lens epithelium-derived growth factor (LEDGF)/
p75
is the dominant binding partner of
HIV
-1 integrase (IN) in human cells. We have determined the NMR structure of the integrase-binding domain (IBD) in LEDGF and identified amino acid residues essential for the interaction. The IBD is a compact right-handed bundle composed of five alpha-helices. Based on folding topology, the IBD is structurally related to a diverse family of alpha-helical proteins that includes eukaryotic translation initiation factor eIF4G and karyopherin-beta. LEDGF residues essential for the interaction with IN were localized to interhelical loop regions of the bundle structure. Interaction-defective IN mutants were previously shown to cripple replication although they retained catalytic function. The initial structure determination of a host cell factor that tightly binds to a retroviral enzyme lays the groundwork for understanding enzyme-host interactions important for viral replication.
...
PMID:Solution structure of the HIV-1 integrase-binding domain in LEDGF/p75. 1589 93
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