Tracking of human cells in mice

Tracking of human cells in mice

Tracking and tracing of transplanted cells in mice is required in many fields of research. Examples are transplantation of stem cells into organs of mice to study their differentiation capacity and injection of tumor cells to examine metastatic behavior. In the present study we tested the lipid dye...

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Veröffentlicht in:Histochemistry and cell biology 2008-08, Vol.130 (2), p.329-338
Hauptverfasser: Schormann, Wiebke, Hammersen, Friedrich J., Brulport, Marc, Hermes, Matthias, Bauer, Alexander, Rudolph, Claudia, Schug, Markus, Lehmann, Thomas, Nussler, Andreas, Ungefroren, Hendrik, Hutchinson, James, Fändrich, Fred, Petersen, Jörg, Wursthorn, Karsten, Burda, Martin R., Brüstle, Oliver, Krishnamurthi, Kannan, von Mach, Marc, Hengstler, Jan G.
Format: Artikel
Sprache:eng
Schlagworte:
Animals
Biochemistry
Biomedical and Life Sciences
Biomedicine
Carbocyanines - chemistry
Carbocyanines - metabolism
Cell Biology
Cell culture
Cell Differentiation
Cell Line, Tumor
Cell Nucleus - chemistry
Cell Nucleus - ultrastructure
Cellular biology
Cord Blood Stem Cell Transplantation
Developmental Biology
Fluorescent Dyes - chemistry
Fluorescent Dyes - metabolism
Humans
In Situ Hybridization, Fluorescence - methods
Lipids
Male
Mice
Mice, Inbred NOD
Mice, SCID
Microscopy, Fluorescence
Nanoparticles
Original Paper
Quantum Dots
Rodents
Transplantation, Heterologous
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Zusammenfassung:Tracking and tracing of transplanted cells in mice is required in many fields of research. Examples are transplantation of stem cells into organs of mice to study their differentiation capacity and injection of tumor cells to examine metastatic behavior. In the present study we tested the lipid dye CM-DiI and red fluorescent nanoparticles Qdot655 for their applicability in tagging and tracing of human cells in mice. Labeling of different cell types, including MCF-7 human breast cancer cells, human cord blood derived cells, human NeoHep cells and human hepatopancreatic precursor cells, is technically easy and did not compromise further cell culture. After transplantation of CM-DiI or Qdot655 marked cells, red fluorescent structures could be detected already in unprocessed paraffin slices of the studied organs, namely liver, lung, pancreas, kidney, spleen and bone marrow. Next, we examined whether the red fluorescent structures represent the transplanted human cells. For this purpose, we established an in situ hybridization (ISH) technique that allows clear-cut differentiation between human and murine nuclei, based on simultaneous hybridization with human alu and mouse major satellite ( mms ) probes. We observed a high degree of coincidence between CM-DiI-marked cells and alu positive nuclei. However, also some mms positive cells contained CM-DiI, suggesting phagocytosis of the transplanted CM-DiI-marked cells. The degree of such CM-DiI-positive mouse cells depended on the cell type and route of administration. From a technical point of view it was important that CM-DiI-positive structures in paraffin slices remained fluorescent also after ISH. In contrast, Qdot655 positive structures faded during further staining procedures. In conclusion, marking of cells with CM-DiI or Qdot655 prior to transplantation facilitates recovery of human cells, since a high fraction of positive structures in the host’s tissue originate from the transplanted cells. However, CM-DiI or Qdot655 positive staining of individual cells in transplanted tissues is not sufficient to prove their human origin. Additional procedures, such as ISH with alu -probes, are essential, when characterizing individual cells.
ISSN:0948-6143
1432-119X
DOI:10.1007/s00418-008-0428-5