Jo Ann Tyndall scite author profile

Jo Ann Tyndall

3Publications

77Citation Statements Received

48Citation Statements Given

How they've been cited

129

How they cite others

Affiliations

The University of Texas Southwestern Medical Center, University of North Carolina at Chapel Hill

Publications

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Polyclonal Antibodies Raised Against Bacillus Calmette-Guerin, Mycobacterium Duvalii, and Mycobacterium Paratuberculosis Used to Detect Mycobacteria in Tissue with the Use of Immunohistochemical Techniques

Wiley

Mulhollan

Beck

et al. 1990

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Commercially available polyclonal antibodies raised against strains of mycobacteria were used to detect organisms in tissue sections from 34 cases of tuberculosis, leprosy, and atypical mycobacteria. Thirty-two cases of fungal infections, granulomatous inflammation, and sarcoidosis were used as negative controls. Sections stained with the use of antibodies raised against Bacillus Calmette-Guerin (BCG), Mycobacterium duvalii (MD), and Mycobacterium paratuberculosis (MP) were compared with Kinyoun and Fite-stained tissue sections. In caseating granulomata, clumps of mycobacterial debris, cells, and cell fragments stained. In histiocytic granulomata of mycobacterial infections, histiocyte cytoplasm contained both organisms and debris. The three antibodies showed cross-reactivity against the four groups of mycobacteria tested. Mycobacterial staining using immunoperoxidase was apparent in most cases at low-power (scanning) magnification. Thirty-two of 34 cases of mycobacterial infection, including all 24 Kinyoun-Fite-positive cases, were positive for immunoreactive organisms and debris using anti-MD, anti-BCG, and/or anti-MP. Eight of ten cases of culture-proven mycobacterial infection, in which Kinyoun and Fite stains were negative, had immunoreactive organisms or antigen with anti-BCG, MD, or MP. The antibodies also stained organisms in five cases of sporotrichosis in which the organisms were identified as yeast forms in tissue sections.

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Structural evidence for leucine at the reactive site of heparin cofactor II

Griffith¹,

Noyes²,

Tyndall³

et al. 1985

Biochemistry

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The reaction products formed during the enzymatic inactivation of heparin cofactor II (HCII) by a proteinase isolated from Echis carinatus were analyzed by sodium dodecyl sulfate (NaDodSO4)-polyacrylamide gel electrophoresis and by reverse-phase high-performance liquid chromatography. By NaDodSO4-polyacrylamide gel electrophoresis, limited proteolysis of HCII was observed, which resulted in a decrease in the apparent molecular weight of the protein from approximately 68 000 to approximately 53 000. By reverse-phase high-performance liquid chromatography, at least 20 peptides were observed. Primary structure analysis of these peptides indicated that significant proteolysis had occurred in the NH2-terminal region of the protein. HCII inactivation, however, coincided with the appearance of a peptide from the COOH-terminal region of the protein. The peptide differed from the previously identified reactive site peptide [Griffith, M. J., Noyes, C. M., & Church, F. C. (1985) J. Biol. Chem. 260, 2218-2225] by only one residue: a leucyl residue at the NH2-terminal of the peptide. We conclude that leucine, as opposed to the expected arginine, is at the reactive site of HCII.

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Enzymatic inactivation of heparin cofactor II by a proteinase (proteinase-1) isolated from venom

Griffith

Tyndall

Noyes

et al. 1985

Thrombosis Research

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Jo Ann Tyndall

Polyclonal Antibodies Raised Against Bacillus Calmette-Guerin, Mycobacterium Duvalii, and Mycobacterium Paratuberculosis Used to Detect Mycobacteria in Tissue with the Use of Immunohistochemical Techniques

Structural evidence for leucine at the reactive site of heparin cofactor II

Enzymatic inactivation of heparin cofactor II by a proteinase (proteinase-1) isolated from venom

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