In search of the skeletal stem cell: isolation and separation strategies at the macro/micro scale for skeletal regeneration
In search of the skeletal stem cell: isolation and separation strategies at the macro/micro scale for skeletal regeneration
Skeletal stem cells (SSCs) show great capacity for bone and cartilage repair however, current in vitro cultures are heterogeneous displaying a hierarchy of differentiation potential. SSCs represent the diminutive true multipotent stem cell fraction of bone marrow mononuclear cell (BMMNC) populations. Endeavours to isolate SSCs have generated a multitude of separation methodologies. SSCs were first identified and isolated by their ability to adhere to culture plastic. Once isolated, further separation is achieved via culture in selective or conditioned media (CM). Indeed, preferential SSC growth has been demonstrated through selective in vitro culture conditions. Other approaches have utilised cell morphology (size and shape) as selection criteria. Studies have also targeted SSCs based on their preferential adhesion to specified compounds, individually or in combination, on both macro and microscale platforms. Nevertheless, most of these methods which represent macroscale function with relatively high throughput, yield insufficient purity. Consequently, research has sought to downsize isolation methodologies to the microscale for single cell analysis. The central approach is identification of the requisite cell populations of SSC-specific surface markers that can be targeted for isolation by either positive or negative selection. SELEX and phage display technology provide apt means to sift through substantial numbers of candidate markers. In contrast, single cell analysis is the paramount advantage of microfluidics, a relatively new field for cell biology. Here cells can be separated under continuous or discontinuous flow according to intrinsic phenotypic and physicochemical properties. The combination of macroscale quantity with microscale specificity to generate robust high-throughput (HT) technology for pure SSC sorting, isolation and enrichment offers significant implications therein for skeletal regenerative strategies as a consequence of lab on chip derived methodology
1206-1220
Gothard, David
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Tare, Rahul S.
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Mitchell, Peter D.
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Dawson, Jonathan I.
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Oreffo, Richard O.C.
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2011
Gothard, David
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Tare, Rahul S.
587c9db4-e409-4e7c-a02a-677547ab724a
Mitchell, Peter D.
a6de2a77-02bc-4679-8717-4ad1153464bd
Dawson, Jonathan I.
b220fe76-498d-47be-9995-92da6c289cf3
Oreffo, Richard O.C.
ff9fff72-6855-4d0f-bfb2-311d0e8f3778
Gothard, David, Tare, Rahul S., Mitchell, Peter D., Dawson, Jonathan I. and Oreffo, Richard O.C.
(2011)
In search of the skeletal stem cell: isolation and separation strategies at the macro/micro scale for skeletal regeneration.
Lab on a Chip, 11 (7), .
(doi:10.1039/C0LC00575D).
(PMID:21350777)
Abstract
Skeletal stem cells (SSCs) show great capacity for bone and cartilage repair however, current in vitro cultures are heterogeneous displaying a hierarchy of differentiation potential. SSCs represent the diminutive true multipotent stem cell fraction of bone marrow mononuclear cell (BMMNC) populations. Endeavours to isolate SSCs have generated a multitude of separation methodologies. SSCs were first identified and isolated by their ability to adhere to culture plastic. Once isolated, further separation is achieved via culture in selective or conditioned media (CM). Indeed, preferential SSC growth has been demonstrated through selective in vitro culture conditions. Other approaches have utilised cell morphology (size and shape) as selection criteria. Studies have also targeted SSCs based on their preferential adhesion to specified compounds, individually or in combination, on both macro and microscale platforms. Nevertheless, most of these methods which represent macroscale function with relatively high throughput, yield insufficient purity. Consequently, research has sought to downsize isolation methodologies to the microscale for single cell analysis. The central approach is identification of the requisite cell populations of SSC-specific surface markers that can be targeted for isolation by either positive or negative selection. SELEX and phage display technology provide apt means to sift through substantial numbers of candidate markers. In contrast, single cell analysis is the paramount advantage of microfluidics, a relatively new field for cell biology. Here cells can be separated under continuous or discontinuous flow according to intrinsic phenotypic and physicochemical properties. The combination of macroscale quantity with microscale specificity to generate robust high-throughput (HT) technology for pure SSC sorting, isolation and enrichment offers significant implications therein for skeletal regenerative strategies as a consequence of lab on chip derived methodology
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Published date: 2011
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Local EPrints ID: 177375
URI: http://eprints.soton.ac.uk/id/eprint/177375
ISSN: 1473-0197
PURE UUID: 27a9bc7b-be1f-4b31-b4b8-89becee59a74
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Date deposited: 17 Mar 2011 10:07
Last modified: 14 Mar 2024 02:53
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David Gothard
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Peter D. Mitchell
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