D. J. Klausner scite author profile

D. J. Klausner

5Publications

3Citation Statements Received

34Citation Statements Given

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University of Minnesota

Publications

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Regulation of mitogen- and antigen-stimulated lymphocyte blastogenesis by prostaglandins

Muscoplat¹,

Klausner²,

Brunner³

et al. 1979

Infect Immun

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Exogenously added prostaglandin El or E2 inhibited the blastogenic response of Mycobacterium bovis-sensitized bovine peripheral blood lymphocytes stimulated with concanavalin A, phytohemagglutinin, or M. bovis purified protein derivative as measured by [3H]thymidine uptake. The kinetics of the response showed that prostaglandins must be added to lymphocyte cultures within hours after mitogen or antigen addition to achieve maximum suppression of [3H]thymidine uptake. Addition of prostaglandins 24 h after the addition of mitogens or antigens resulted in considerably less suppression, supporting a hypothesis that prostaglandins initiate an early series of events which ultimately control lymphocyte blastogenesis rather than directly inhibit deoxyribonucleic acid synthesis.

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Development of a whole blood lymphocyte stimulation assay for detecting hypersensitivity to PPD in cattle experimentally infected with Mycobacterium bovis

Muscoplat

Johnson

Thoen

et al. 1977

Veterinary Microbiology

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Whole-blood lymphocyte stimulation assay for measurement of cell-mediated immune responses in bovine brucellosis

Kaneene¹,

Anderson²,

Johnson³

et al. 1978

J Clin Microbiol

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A study was conducted to develop an in vitro whole-blood lymphocyte stimulation assay for measurement of cell-mediated immune response in bovine brucellosis. A soluble antigen (BASA) prepared from killed cells of Brucella abortus 1119-3 was used. Cattle infected with B. abortus field strains, B. abortus 19 calfhood- and adult-vaccinated cattle, and nonexposed cattle were tested. Blood was diluted 10-fold in RPMI-1640 medium (without added serum) and cultured with BASA (at a concentration of 2.2 microgram per culture) at varying times of incubation. Results were assayed for [3H]thymidine incorporation into deoxyribonucleic acid. A 6-day period was found to be optimal for incubating blood cultures to achieve maximum specific lymphocyte stimulation. Serological tests and bacteriological isolation attempts were conducted simultaneously with lymphocyte stimulation tests, and there was a significant correlation between cell-mediated immune response and bacteriological findings. There was a significant correlation between cell-mediated immune response and the level of serum antibodies on a group basis, but there was little correlation between the two systems on individual infected animals. Among vaccinated animals there was little or no correlation between cell-mediated immune and humoral responses. The whole-blood assay was found to be simple, fast, sensitive, and reproducible.

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In vitro stimulation of bovine peripheral blood lymphocytes: comparison of round- and flat-bottom microtiter plates for detection of tuberculin hypersensitivity

Sloane¹,

Muscoplat²,

Kaneene³

et al. 1978

J Clin Microbiol

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Lymphocytes from Mycobacterium bovis-sensitized and normal cattle were cultured in round- and/or flat-bottom microtiter plates and stimulated with M. bovis purified protein derivative (PPD) tuberculin. Blastogenic responses of lymphocytes from M. bovis-sensitized cattle to PPD cultured in round-bottom plates were significantly greater than those of lymphocytes cultured in flat-bottom microtiter plates. Normal lymphocytes of nonsensitized cattle were not stimulated by PPD in either round- or flat-bottom microtiter plates. Kinetics of lymphocyte responses in round-bottom plates are presented.

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Kinetics of levamisole-induced potentiation of lymphocyte blastogenic responses inMycobacterium bovis sensitized lymphocyties

et al. 1979

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A study was conducted to determine the kinetics of levamisole-induced potentiation of lymphocyte blastogenesis in Mycobacteriumbovis sensitized and nonsensitized cattle lymphocytes. It was observed that levamisole significantly potentiated PPDinduced blastogenic responses when it (levamisole) was added to M.~ boris sensitized lymphocyte cultures 24 hours prior to the addition of PPD. Levamisole-indueed either minimal or suppressed the PPD-induced lymphocyte stimulation response in M. boris nonexposed control lymphocytes. The implications of~ossib!e use of levamisole in cellular in vitro assays for studying anergy or general unresponsiveness are discussed.

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D. J. Klausner

Regulation of mitogen- and antigen-stimulated lymphocyte blastogenesis by prostaglandins

Development of a whole blood lymphocyte stimulation assay for detecting hypersensitivity to PPD in cattle experimentally infected with Mycobacterium bovis

Whole-blood lymphocyte stimulation assay for measurement of cell-mediated immune responses in bovine brucellosis

In vitro stimulation of bovine peripheral blood lymphocytes: comparison of round- and flat-bottom microtiter plates for detection of tuberculin hypersensitivity

Kinetics of levamisole-induced potentiation of lymphocyte blastogenic responses inMycobacterium bovis sensitized lymphocyties

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