Newly recognized rat parvoviruses : characterization and diagnostic assay development /

Wan, Zhuohua,

January 2001

Thesis (Ph. D.)--University of Missouri--Columbia, 2001. / "May 2001." Typescript. Vita. Includes bibliographical references (leaves 85-89). Also available on the Internet.

Newly recognized rat parvoviruses characterization and diagnostic assay development /

Wan, Zhuohua,

January 2001

Thesis (Ph. D.)--University of Missouri--Columbia, 2001. / Typescript. Vita. Includes bibliographical references (leaves 85-89). Also available on the Internet.

Differentiating between living and non-living prokaryotic cells : development, evaluation, and application of a modified vital stain and probe method (mVSP)

Howard-Jones, Michelle Hope

08 1900

No description available.

Bacteriology Technique

Bacteria

Microbiological assay

I. Development of a new assay and inhibitors for human cystathionine beta-synthase II. Asymmetric catalyst development guided by in situ enzymatic screening (ISES) /

Shen, Weijun.

January 1900

Thesis (Ph.D.)--University of Nebraska-Lincoln, 2007. / Title from title screen (site viewed Aug. 1, 2007). PDF text: 292 p. : ill. (some col.) UMI publication number: AAT 3256642. Includes bibliographical references. Also available in microfilm and microfiche formats.

Assessment of the effect of dosing regime and cell culture model on micronucleus induction in in vitro genotoxicity test systems

Chapman, Katherine Emma

January 2015

No description available.

616

A filter paper assay for low cellulase activities and the cultivation of Trichoderma reesei on acid whey and sweet whey permeate

Nordmark, Tor Soren

24 November 1993

The traditional filter paper assay for saccharifying cellulase originally described by M. Mandels et al (1976) has been modified to make possible low activity determinations of Trichoderma cellulases. The enzymatic activity appears to decline during a prolonged incubation period if no precautions have been taken. By means of adding bovine serum albumin and potassium chloride as protein stabilizers and sodium azide as an antimicrobial agent filter paper activities in the range from 0.02 to 0.37 (IUPAC assay, 1987) can be estimated by extending the incubation time up to 20 hours. Filter paper activity values obtained by this method may be compared to those obtained by the IUPAC assay by using a conversion factor from 1.4 to 1.7. Acid whey and sweet whey permeate have been investigated as media for growth and metabolite production by Trichoderma reesei QM 9414 using shake flask cultures and spore inocula. In the case of acid whey the mycelial growth after 2 weeks is 13 mg dry weight /ml substrate. The specific growth rate is 0.29/day. The fungus appears to metabolize the whey protein the first 2 weeks. The alkalinity of acid whey rises continuously over a three week period up to a pH of 8.5. In the case of whey permeate the maximal mycelial weight gain is 4.4 mg/ml which appears after 8 days. A rise in net soluble protein level comes after 3-5 days and reaches a maximum value of 0.23 mg/ml after 2 weeks. The pH of whey permeate rises continuously to 7.5 after 3 days and then slowly declines. The net production of cellulases is low on both media. Dilution 1:6 of the acid whey, supplementation with ammonium sulfate and pHadjustments did not enhance the production of cellulases. Acid whey supports a significant growth and sweet whey permeate shows potential for extracellular protein production. A literature review surveys the composition and uses of acid whey, environmental aspects of whey wastes, the fungus Trichoderma reesei, the mode of action of the Trichoderma reesei cellulase system and the structure of cellulose in cotton and wood. / Graduation date: 1994

Microbiological assay

Trichoderma reesei

Filters and filtration

Whey

Rapid assay for Bacillus proteinases in raw milk as detected by a simple casein denaturation method

Feijoo, Sergio C.

09 January 1991

A casein agar diffusion method was developed to detect and quantify pertinent levels of proteinases produced in raw milk supplies by heat resistant Bacillus sporeformers. In order to optimize the required heat treatment conditions of raw milk samples, trials that involved a combination of different temperatures and times were evaluated. A heat treatment of 75°C for 20 min was the most effective for recovering the highest number of surviving spores. A sporulation broth containing five different minerals and supplemented with 0.2% nonfat dry milk was used to maximize spore production in all heat-treated samples. A β-casein based assay detected proteinase activity from raw milk samples that ranged from 0.093 to 4.034 units/mg which corresponded to zones of β-casein precipitation in the β-casein agar of 5.0 and 15.0 mm respectively, and was compared to Protease Type VIII (from B. licheniformis). This assay correlated well with the fluorescein isothiocyanate casein-labeled assay (FITC), R=0.995 (Protease Type VIII). Proteases of Bacillus origin such as Protease Type IX, X, XV and XXXI were also evaluated but were rejected in favor of a broader range of activity expressed by Protease Type VIII. For an initial set of 370 raw milk samples, no quality deterioration, such as coagulation or bitter taste was observed in heat-treated (75°C for 20 min) and incubated samples (7.2°C for 10 days). However, during the winter season, 18 of 75 incubated samples (7.2°C for 10 days) tasted slightly bitter and exhibited a slight degree of casein precipitation. One sample coagulated but exhibited no proteinase activity on the β-casein agar gel, hence it was considered a false negative. The positive results for proteinase activity from raw Grade A samples tested by the β-casein agar diffusion method did not correlate either with fresh spore counts (R=0.21) or post-heat treatment incubation counts (R=0.03) or with psychrotrophic sporeformer counts (R=0.06). The β-casein agar diffusion method is simple, rapid and sensitive to Bacillus spp. proteinases, but was unreliable in projecting results related to the psychrotrophic sporeformer count. Consequently, further research is required to establish optimum conditions (time and/or temperature) and inoculum volumes into sporulation broth for attainment of a more positive correlation between β-casein agar precipitation zones and psychrotrophic sporeformer populations of either raw or processed milk samples. / Graduation date: 1991

Microbiological assay

Milk

Proteins -- Denaturation

Bacillus (Bacteria)

Modified limiting dilution analysis : a mathematical model with biological interpretation

Maier, Stefan H.

04 April 1994

A mathematical model of Limiting Dilution Analysis for two limiting parameters is presented and investigated. Limiting Dilution Analysis is a microbiological cell assay developed for immunological application. In the given case we deal with the interaction between B lymphocytes, macrophage derived factor and T-independent antigens. The state of the art is that quantitative statements are only possible if one cell type (in general the B cells) is limiting and all others are in excess present. The basis for this thesis is a set of experiments in which B cells and macrophage derived factor are limiting and all other involved cells and factors are in saturating amounts present. It is shown that so far presented suggestions on modeling Limiting Dilution Analysis for two limiting cell-types are not suitable for this problem. Further, a mathematical model based on data is presented and interpreted in immunological terms with the help of a set of partial differential equations. The basis for the interpretation of the model are changes in affinity and saturation effects, both not incorporated in the so far presented models of the assay. In particular the relevance of mathematical interpretation of this process for the identification of new concepts as the saturation effects is stressed. The model of partial differential equations is highly non-linear but offers the possibility of interpreting the highly interrelated processes apart from each other. / Graduation date: 1994

Immunoassay -- Mathematical models

Development of a field-based assay for rapid detection of enterohemorrhagic Escherichia coli (EHEC)

Willford, John Daniel.

January 2008

Thesis (Ph.D.)--University of Wyoming, 2008. / Title from PDF title page (viewed on August 5, 2009). Includes bibliographical references (p. 123-138).

Development of an in vitro assay for MMP cleavage

Wu, Wing-kei, Ricky., 胡永基.

January 2005

published_or_final_version / Medical Sciences / Master / Master of Medical Sciences

Metalloproteinases.

Extracellular matrix proteins.

Microbiological assay.