Quantitative Determination of Lentiviral Vector Particle Numbers by Real-Time PCR | Zendy

Michaela Scherr | Zendy; Karin Battmer | Zendy; Ulrike Blömer | Zendy; Arnold Ganser | Zendy; Manuel Grez | Zendy

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Quantitative Determination of Lentiviral Vector Particle Numbers by Real-Time PCR

Author(s) -

Michaela Scherr,

Karin Battmer,

Ulrike Blömer,

Arnold Ganser,

Manuel Grez

Publication year - 2001

Publication title -

biotechniques

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 0.617

H-Index - 131

eISSN - 1940-9818

pISSN - 0736-6205

DOI - 10.2144/01313st05

Subject(s) - vector (molecular biology) , real time polymerase chain reaction , viral vector , complementary dna , virology , microbiology and biotechnology , dna , biology , computational biology , capsid , virus , recombinant dna , genetics , gene

Here, we describe a quantitative, DNA-based, real-time PCR approach to determine the number of lentivirus particles that are present in vector preparations. In this approach, the minus strong-stop cDNA fragment that is present in viral capsids serves as template for PCR. Using this technology, we found that only 0.1%-1% of the virus particles that are present in vector preparations are infectious. The approach described here is rapid, reliable, and simple in concept and can be used to estimate both vector particles in supernatants and the number of infectious particles. Also, this approach can easily be adapted to a high-throughput system by using 96-well plates and a 2-h running time.

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