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Dive into the research topics where William V. Burnett is active.

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Featured researches published by William V. Burnett.


Cancer Immunology, Immunotherapy | 1990

Antibody-penicillin-V-amidase conjugates kill antigen-positive tumor cells when combined with doxorubicin phenoxyacetamide

David Kerr; Peter D. Senter; William V. Burnett; David L. Hirschberg; Ingegerd Hellström; Karl Erik Hellström

SummaryThe two monoclonal antibodies (mAb), L6 (anti-carcinoma), and 1F5 [anti-(B-cell-lymphoma)], were chemically linked to the enzyme penicillin-V amidase (PVA), which hydrolyzes phenoxyacetamides, to explore the potential of using mAb-enzyme conjugates for the localizaton of chemotherapeutic drugs at tumor cells. The phenoxyacetamide derivatives of doxorubicin and melphalan were prepared, yielding the less toxic amides, doxorubicin-N-p-hydroxyphenoxyacetamide (DPO) and melphalan-N-p-hydroxyphenoxyacetamide (MelPO). These were hydrolyzed by PVA to doxorubicin and melphalan respectively.In vitro studies with the L6-positive lung carcinoma cell line, H2981, and the 1F5-positive B-cell lymphoma line, Daudi, showed that DPO was 80-fold less toxic to H2981 cells and 20-fold less toxic to Daudi cells than doxorubicin, and its toxicity was substantially increased when the H2981 cells were pretreated with L6-PVA or the Daudi cells were pretreated with 1F5-PVA. The cytotoxic effect was antigen-specific, since only the binding mAb-enzyme conjugate increased the cytotoxicity of the prodrug. MelPO was more than 1000-fold less toxic than melphalan to H2981 cells and more than 100-fold less toxic than melphalan to Daudi cells. Pretreatment with the mAb-PVA conjugates did not enhance the toxicity of MelPO in either cell line, because PVA hydrolyzes the phenoxyacetamide bond of MelPO too slowly to generate a toxic level of melphalan.


Biotechnology Letters | 1987

Bifunctional cosmid vector forStreptomyces

Julia J. Portmore; William V. Burnett; Shu-Jen Chiang

SummaryAnEscherichiacoli/Streptomyces bifunctional cosmid vector, pJP3, which selects for clones with insert size 23–33 kilobase pairs (kb), has been constructed. A genomic DNA library fromS.kanamyceticus has been stably maintained inE.coli using pJP3. This recombinant DNA can be transferred intoS.lividans with increased efficiency by utilizing heat treatment during protoplast formation.


Archive | 2003

Mammalian cell culture processes for protein production

Bernhard M. Schilling; Linda Matlock; Stephen G. Zegarelli; William V. Burnett; Christoph E. Joosten; Jonathan D. Basch; Steven S. Lee


BioTechniques | 1997

Northern blotting of RNA denatured in glyoxal without buffer recirculation.

William V. Burnett


Applied and Environmental Microbiology | 1997

Purification and characterization of a cephalosporin esterase from Rhodosporidium toruloides.

Michael Politino; Sean M. Tonzi; William V. Burnett; Guna Romancik; John J. Usher


Archive | 2009

Mammallian cell culture process for protein production

Bernhard M. Schilling; Linda Matlock; Stephen G. Zegarelli; William V. Burnett; Christoph E. Joosten; Jonathan D. Basch; Steven S. Lee


Archive | 2001

Glutaryl cephalosporin amidase from pseudomonas diminuta bs-203

Ross Binder; Joanne L. Brown; Thomas J. Franceschini; William V. Burnett; Michael Politino; Suo Win Liu; Sean M. Tonzi


Archive | 1997

Cephalosporin esterase gene from Rhodosporidium toruloides

Michael Politino; Sean M. Tonzi; John J. Usher; William V. Burnett; Guna Romancik


Archive | 2003

Verfahren zur kultivierung vonsäugetierzellen zur proteinproduktion

Jonathan D. Basch; William V. Burnett; Christoph E. Joosten; Steven S. Lee; Linda Matlock; Bernhard M. Schilling; Stephen G. Zegarelli


Archive | 2003

Processus de culture de cellules de mammiferes pour la production de proteines

Bernhard M. Schilling; Linda Matlock; Stephen G. Zegarelli; William V. Burnett; Christoph E. Joosten; Jonathan D. Basch; Steven S. Lee

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