Hybridization immune deficiency virus strain and application
An immunodeficiency virus, virus strain technology, applied in the direction of virus/bacteriophage, medical preparations containing active ingredients, antibody medical ingredients, etc., can solve the problem that the natural infection state of HIV-1 cannot be well simulated.
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Embodiment 1
[0086] Construction of SHIV, SHIV-B' against the main epidemic strain HIV-1B' subtype in central China WHU Should carry the outer membrane gene (env) of representative B' subtype HIV-1.
[0087] In order to understand that the HIV-1 selected for SHIV construction is the B' subtype strain, early HIV-102HNsmx2 was isolated from an HIV-infected patient in Henan, and the tat / rev of HIV-102HNsmx2 was amplified from the cell genome by PCR / vpu / env gene sequence, its sequencing. Molecular analysis of the tat / rev / vpu / env genotype of HIV-102HNsmx2 and how it differs from other HIV-1 strains.
[0088] Isolation and culture of peripheral blood mononuclear cells (PBMC) from HIV-1 infected patients and healthy individuals:
[0089] 1. Obtain whole blood (heparin anticoagulated) from HIV-1 infected persons (02HNsmx2) and healthy persons, process or detect tissues, body fluids or excreta that have been separated from the human body or organism to obtain information as an intermediate resul...
Embodiment 2
[0117] HIV-1 02HNsmx2 tat / rev / vpu / env reading frame integrity and genotype of R5 tropism.
[0118] In order to prove that the open reading frame of each gene of HIV-1 02HNsmx2 tat / rev / vpu / env is complete and has the ability to express proteins in vivo and in vitro, its gene sequence was analyzed to rule out the possibility of not having a complete reading frame. It is necessary to construct an R5-tropic SHIV, so the phenotype of HIV-102HNsmx2 env must be proved to be R5-tropic before constructing SHIV.
[0119] Analysis of HIV-1 02HNsmx2 tat / rev / vpu / env gene reading frame:
[0120] The entire tat / rev / vpu / env gene sequence of HIV-1 02HNsmx2 was compared with the corresponding sequence of the standard strain HIV-1 HXB2 using the ClustalX1.81 program, and the sequence after comparison was submitted to the HIV Databases website ( www.hiv-web.lanl.gov / content / index ). After clicking the Gene Cutter of Tool, the website analyzes the open reading frames of the tat, rev, vpu and en...
Embodiment 3
[0126] Construction of hybrid virus strain SHIV-B' WHU .
[0127] In order to obtain the hybrid virus strain SHIV-B' WHU , the applicant first cloned the 3' end vector carrying the HIV-1B' tat / rev / vpu / env gene, and the vector and the 5' end plasmid were co-transfected into 293T cells to construct a hybrid virus.
[0128] Construction of 3' chimeric vector (3'-p02HN SMX2 -B' WHU ):
[0129] 1. Digest the HIV-1 tat / rev / vpu / env gene fragment from p2'ENV-VAX with restriction enzymes SphI and XhoI, and use the gel recovery kit to recover the exogenous HIV-1 tat / rev / vpu / env gene (3Kb). 3' end vector (3'-pvpu + ) is a non-expression vector (Chen, Z., et al., 2000.Enhanced Infectivity of an R5-Tropic Simian / Human Immunodeficiency Virus Carrying Human Immunodeficiency Virus Type 1 Subtype C Envelope after Serial Passages in Pig-Tailed Macaques (Macaca nemestrina). J Virol, 74: 6501-6510). Digest vector 3'-pvpu with restriction enzymes SphI and XhoI + and dephosphorylated.
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