1. Determining the minimum number of detectable cardiac-transplanted111In-tropolone-labelled bone-marrow-derived mesenchymal stem cells by SPECT
- Author
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Peter Merrifield, Huafu Kong, Frank S. Prato, Yuan Jin, Rob Z Stodilka, Jane Sykes, R. Glenn Wells, and Pamela Zabel
- Subjects
Cell Survival ,Bone Marrow Cells ,Mesenchymal Stem Cell Transplantation ,Tropolone ,Imaging phantom ,chemistry.chemical_compound ,Dogs ,medicine ,Animals ,Radiology, Nuclear Medicine and imaging ,Viability assay ,Cells, Cultured ,Cell Proliferation ,Radiological and Ultrasound Technology ,Phantoms, Imaging ,business.industry ,Cell growth ,Indium Radioisotopes ,Mesenchymal stem cell ,Heart ,Mesenchymal Stem Cells ,Transplantation ,medicine.anatomical_structure ,chemistry ,Bone marrow ,Stem cell ,Nuclear medicine ,business - Abstract
In this work, we determined the minimum number of detectable 111In-tropolone-labelled bone-marrow-derived stem cells from the maximum activity per cell which did not affect viability, proliferation and differentiation, and the minimum detectable activity (MDA) of 111In by SPECT. Canine bone marrow mesenchymal cells were isolated, cultured and expanded. A number of samples, each containing 5x10(6) cells, were labelled with 111In-tropolone from 0.1 to 18 MBq, and cell viability was measured afterwards for each sample for 2 weeks. To determine the MDA, the anthropomorphic torso phantom (DataSpectrum Corporation, Hillsborough, NC) was used. A point source of 202 kBq 111In was placed on the surface of the heart compartment, and the phantom and all compartments were then filled with water. Three 111In SPECT scans (duration: 16, 32 and 64 min; parameters: 128x128 matrix with 128 projections over 360 degrees) were acquired every three days until the 111In radioactivity decayed to undetectable quantities. 111In SPECT images were reconstructed using OSEM with and without background, scatter or attenuation corrections. Contrast-to-noise ratio (CNR) in the reconstructed image was calculated, and MDA was set equal to the 111In activity corresponding to a CNR of 4. The cells had 100% viability when incubated with no more than 0.9 MBq of 111In (80% labelling efficiency), which corresponded to 0.14 Bq per cell. Background correction improved the detection limits for 111In-tropolone-labelled cells. The MDAs for 16, 32 and 64 min scans with background correction were observed to be 1.4 kBq, 700 Bq and 400 Bq, which implies that, in the case where the location of the transplantation is known and fixed, as few as 10,000, 5000 and 2900 cells respectively can be detected.
- Published
- 2005
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