CD31(-) HipOps - A Highly Osteogenic Cell Population From Mouse Bone Marrow

McKenzie, Kristen Penny

04 December 2012

Multipotent mesenchymal stem cells (MSCs), found in many adult tissues, may be useful for regenerative medicine applications. Their identification and purification have been difficult due to their low frequency and lack of unambiguous markers. Using a magnetic micro-beads negative selection technique to remove contaminating hematopoietic cells from mouse bone marrow stromal cells (BMSCs), our lab recently isolated a highly purified osteoprogenitor (HipOp) population that was also enriched for other mesenchymal precursors, including MSCs (Itoh and Aubin, 2009). To further enhance enrichment, we positively selected BMSCs and HipOps for CD73, a putative MSC marker, which resulted in no significant additional enrichment for osteoprogenitors when the population was tested in vitro. However, we also found that HipOps were enriched in vascular endothelial cells, and that removing these cells by further negative selection with CD31/PECAM resulted in a CD31(-) HipOp population with higher osteogenic capacity than HipOps in vitro and in vivo.

mesenchymal stem cell

osteoprogenitor

osteoblast

MACS

magnetic bead cell sorting

cell sorting

osteogenesis

CD31

PECAM

cell culture

negative selection

cell marker

bone marrow stromal cell

BMSC

HipOp

bone marrow

vascular endothelial cell

limiting dilution analysis

accessory population

CD73

0379

Studies on Isolation and Identification of Clostridium botulinum Investigating Field Samples Specially from Equine Grass Sickness Cases / Studies on Isolation and Identification of Clostridium botulinum Investigating Field Samples Specially from Equine Grass Sickness Cases

Saeed, Elhassan Mohammed Ali

03 February 2005

No description available.

630 Landwirtschaft

Veterinärmedizin

Agricultural Sciences

Equine grass sickness

Botulismus

C. botulinum

C.tetani

C. perfringens

E. coli

Mäuse-Bioassay

Pferde

Rinder

Geflügel

MB-ELISA

PCR

Equine grass sickness

botulism

C. botulinum

C.tetani

C. perfringens

E. coli

horses

cattle

chicken

mouse bioassay

PCR

Bakteriologie

Review of magnetic bead surface markers for stem cell separation : Literature study for MAGic Bioprocessing

Holmberg, Gustav, Svensson, Adrian, Bergström, Erik, Westerberg, Leo, Wijitchakhorn, Watthachak

January 2022

Stem cell therapy and transplantation is a quickly evolving field with many clinical applications. However, several problems need to be overcome before they can be applied on an allogenic scale, and among them is ensuring of the purity of the applied differentiated stem cell culture. Separation using magnetic beads which attach to the wanted cells has proven to be an effective and easy method to separate them from a sample. An important factor with the method is the choice of specific surface antigens on the beads which determines how well the beads are attached to the cell.  This report will provide some fact of the immunotherapy and some of the most important stem cells and their differentiation to an active cell. It will be elucidated which cytokines are important for differentiation, and current clinical studies in the immunotherapeutic field of stem cells and their useful surface antigens. Furthermore, regenerative medicine using stem cells will be covered. A brief overview mesenchymal and induced pluripotent stem cells, their biological markers, and their various uses. Specific projects using regenerative medicine will be described and an overview of ever-expanding market for regenerative medicine will also be included.

Magnetic bead

stem cell

surface antigen

immunotherapy

regenerative medicine

market analysis

separation technique

Chemical Engineering

Kemiteknik

Biomedical Laboratory Science/Technology

Engineering antibodies to study and improve immunomagnetic isolation of tumour cells

Jain, Jayati

January 2013

Cell separation based on antibody-targeted magnetic beads has been widely used in a number of applications in immunology, microbiology, oncology and more recently, in the isolation of circulating tumour cells (CTCs) in cancer patients. Although other cell separation techniques such as size based cell filtration and Fluorescence Activated Cell Sorting have also been in popular use, immunomagnetic cell isolation possesses the advantages of high throughput, good specificity and reduced cell stress. However, certain fundamental features of the cell-bead interface are still unknown. In this study, some of the key features of the cell-bead synapse were investigated in an effort to improve the efficiency of immunomagnetic cell isolation and reduce its dependence on high expressing cell surface markers. A clinically relevant antibody fragment (Fab) against tyrosine kinase receptor HER2 was applied to study the immunomagnetic isolation of HER2 expressing cancer cells. First, the minimum number of target proteins required on a cell for it to be isolated was determined. Second, the importance of the primary antibody affinity was investigated, using a series of Fab mutants with known kinetics and it was shown that despite starting with sub-nanomolar affinity, improving Fab affinity increased cell isolation. Third, the influence of the connection between the primary antibody and the bead was studied by comparing Fab bridged to the magnetic bead via a secondary antibody, Protein L or streptavidin; the high affinity biotin-streptavidin linkage increased isolation sensitivity by an order of magnitude. Fourth, the effect of manipulating cytoskeletal polymerization and cell membrane fluidity using small molecules was tested; cholesterol depletion decreased isolation and cholesterol loading increased cell isolation. The insights from these observations were then applied to isolate a panel of cell lines expressing a wide range of surface HER2. While the standard approach isolated less than 10% of low HER2 expressing cancer cells from spiked rabbit and human blood, our enhanced approach with the optimized cholesterol level, antibody affinity and antibody-bead linkage could specifically isolate more than 80% of such cells. The final part of this work focussed on developing an antibody clamp that could physically restrict the antigen within its binding site on the Fab and prevent antigen dissociation, using the HER2-Fab complex and the anti-myc peptide antibody 9E10. Work from this thesis provides useful insights into the molecular and cellular parameters guiding immunomagnetic cell isolation and can be used to extend the range of target receptors and biomarkers for tumour cell isolation and other types of cell separation, thereby enhancing the power and capacity of this approach.

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