Analysis of Human Immunodeficiency Virus Type 1 Integration by Using A Specific, Sensitive and Quantitative Assay Based on Real-time Polymerase Chain Reaction

Yamamoto, Norio; Tanaka, Chika; Wu, Yixuan; Chang, Myint Oo; Inagaki, Yutaka; Saito, Yasunori; Naito, Toshio; Ogasawara, Hitoshi; Sekigawa, Iwao; Hayashida, Yasuo

doi:10.1007/s11262-005-5851-2

Cited by 50 publications

(39 citation statements)

References 24 publications

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“…Real-time PCR experiments were performed as described in ref. 45. The second round of PCR was performed on 1/25 of the first-round PCR product in a mixture containing 300 nM each primer, 12.5 l of 2ϫ SYBR green master mix (Applied Biosystems) at a final volume of 25 l, run on an ABI PRIZM 7700 (Applied Biosystems).…”

Section: Methodsmentioning

confidence: 99%

Inhibiting HIV-1 integrase by shifting its oligomerization equilibrium

Hayouka

Rosenbluh²,

Levin³

et al. 2007

Proc. Natl. Acad. Sci. U.S.A.

172

200

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Proteins are involved in various equilibria that play a major role in their activity or regulation. The design of molecules that shift such equilibria is of great therapeutic potential. This fact was demonstrated in the cases of allosteric inhibitors, which shift the equilibrium between active and inactive (R and T) states, and chemical chaperones, which shift folding equilibrium of proteins. Here, we expand these concepts and propose the shifting of oligomerization equilibrium of proteins as a general methodology for drug design. We present a strategy for inhibiting proteins by ''shiftides'': ligands that specifically bind to an inactive oligomeric state of a disease-related protein and modulate its activity by shifting the oligomerization equilibrium of the protein toward it. We demonstrate the feasibility of our approach for the inhibition of the HIV-1 integrase (IN) protein by using peptides derived from its cellularbinding protein, LEDGF/p75, which specifically inhibit IN activity by a noncompetitive mechanism. The peptides inhibit the DNA-binding of IN by shifting the IN oligomerization equilibrium from the active dimer toward the inactive tetramer, which is unable to catalyze the first integration step of 3 end processing. The LEDGF/ p75-derived peptides inhibit the enzymatic activity of IN in vitro and consequently block HIV-1 replication in cells because of the lack of integration. These peptides are promising anti-HIV lead compounds that modulate oligomerization of IN via a previously uncharacterized mechanism, which bears advantages over the conventional interface dimerization inhibitors.allostery ͉ protein equilibrium ͉ shiftides ͉ peptides ͉ drug design

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Section: Methodsmentioning

confidence: 99%

Inhibiting HIV-1 integrase by shifting its oligomerization equilibrium

Hayouka

Rosenbluh²,

Levin³

et al. 2007

Proc. Natl. Acad. Sci. U.S.A.

172

200

View full text Add to dashboard Cite

show abstract

“…21 Briefly, Integrated HIV-1 sequences were amplified by two PCR replication steps using the HIV-1 LTR-specific primer (LTR-TAG-F 5'-ATG CCA CGT AAG CGA AAC TCT GGC TAA CTA GGG AAC CCA CTG-3') and Alu-targeting primers (first-Alu-F 5'-AGC CTC CCG AGT AGC TGG GA-3' and first-Alu-R 5'-TTA CAG GCA TGA GCC ACC G-3'). 52 Alu-LTR fragments were amplified from 10 ng of total cell DNA in a 25-µl reaction mixture containing 1X PCR buffer, 3.5 mM MgCl 2 , 200 µM dNTPs, 300 nM primers, and 0.025 units/µl of Taq polymerase. The first-round PCR cycle conditions were as follows: a DNA denaturation and polymerase activation step of 10 min at 95°C and then 12 cycles of amplification (95°C five washes with PBS + 0.05% Tween 20 between antibodies.…”

Section: 49mentioning

confidence: 99%

Nucleocytoplasmic shuttling of HIV-1 integrase is controlled by the viral Rev protein

Levin¹,

Hayouka²,

Friedler³

et al. 2010

Nucleus

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“…AMs were infected with HIV-1 JRFL, as described previously here, and DNA was extracted from the AMs after 72 hours with the Dneasy Tissue Kit (Qiagen). A two-step nested amplification was performed to initially amplify sequences exclusively containing only human 300-base pair repetitive DNA sequences (Alu) adjacent to HIV-1 envelope, based on a recently published method (34). Primers and probes were developed to quantify human Alu sequences and the JRFL envelope gene with the PrimerExpress software (Perkin Elmer).…”

Section: Taqman Real-time Pcr Analysis Of Chromosomally Integrated Himentioning

confidence: 99%

Adenovirus Vectors Block Human Immunodeficiency Virus–1 Replication in Human Alveolar Macrophages by Inhibition of the Long Terminal Repeat

Kaner

Santiago²,

Rahaghi³

et al. 2010

Am J Respir Cell Mol Biol

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Analysis of Human Immunodeficiency Virus Type 1 Integration by Using A Specific, Sensitive and Quantitative Assay Based on Real-time Polymerase Chain Reaction

Cited by 50 publications

References 24 publications

Inhibiting HIV-1 integrase by shifting its oligomerization equilibrium

Inhibiting HIV-1 integrase by shifting its oligomerization equilibrium

Nucleocytoplasmic shuttling of HIV-1 integrase is controlled by the viral Rev protein

Adenovirus Vectors Block Human Immunodeficiency Virus–1 Replication in Human Alveolar Macrophages by Inhibition of the Long Terminal Repeat

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