Optimized localization of bacterial infections with technetium-99m labelled human immunoglobulin after protein charge selection

To improve the scintigraphic detection of bacterial infections a protein charge-purified fraction of polyclonal human immunoglobulin was applied as a radiopharmaceutical. This purification was achieved by attaching the immunoglobulin to an anion-exchanger column and by obtaining the column-bound fra...

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Bibliographic Details
Published in:European Journal of Nuclear Medicine 1994-10, Vol.21 (10), p.1135-1140
Main Authors: WELLING, M, FEITSMA, H. I. J, CALAME, W, ENSING, G. J, GOEDEMANS, W, PAUWELS, E. K. J
Format: Article
Language:English
Subjects:
Animals
Biological and medical sciences
Humans
Immunoglobulins
Investigative techniques, diagnostic techniques (general aspects)
Klebsiella Infections - diagnostic imaging
Klebsiella pneumoniae
Male
Medical sciences
Mice
Miscellaneous. Technology
Radioimmunodetection - methods
Radionuclide investigations
Specific Pathogen-Free Organisms
Staphylococcal Infections - diagnostic imaging
Technetium
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Summary:To improve the scintigraphic detection of bacterial infections a protein charge-purified fraction of polyclonal human immunoglobulin was applied as a radiopharmaceutical. This purification was achieved by attaching the immunoglobulin to an anion-exchanger column and by obtaining the column-bound fraction with buffer. The binding to bacteria in vitro and the target to non-target ratios of an experimental thigh infection with Staphylococcus aureus or Klebsiella pneumoniae in mice were evaluated to compare the purified and the unpurified immunoglobulin. The percentage of binding to all gram-positive and gram-negative bacteria used in this study was significantly (P < 0.03) higher for the purified than for the unpurified immunoglobulin. For the in vivo study, mice were infected in the thigh muscle with Staph. aureus or K. pneumoniae. After 18 h 0.1 mg of technetium-99m labelled polyclonal immunoglobulin or 99mTc-labelled protein charge-purified polyclonal human immunoglobulin was administered intravenously. At all time intervals the target (infected thighs) to non-target (non-infected thighs) ratios for both infections were significantly higher (P < 0.03) for protein charge-purified polyclonal immunoglobulin than for unpurified polyclonal human immunoglobulin. Already within 1 h the infected tissues could be detected by the purified immunoglobulin. It is concluded that 99mTc-labelled protein charge-purified immunoglobulin localizes both a gram-positive and a gram-negative thigh infection more intensely and faster than 99mTc-labelled unpurified immunoglobulin.
ISSN:0340-6997
1619-7089
DOI:10.1007/BF00181070