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Last Updated: March 29, 2024

Claims for Patent: 10,131,880


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Summary for Patent: 10,131,880
Title:Pluripotent human adipose adult stem cells: isolation, characterization and clinical implications
Abstract: Methods for the efficient isolation and use of pluripotent adipose-derived stem cells (PASCs) are provided. In certain embodiments the methods involve providing an adipose tissue sample from which the stromal vascular fraction is co-cultured with the adipocyte fraction. PASCs can be isolated with a high degree of purification without requiring an additional cell enrichment process (e.g. cell sorting). PASCs and their conditioned media can be used for tissue regeneration within hours of harvesting the adipose tissue, and without requiring cell expansion. PASCs can grow as floating individual cells, as clusters of cells, or attached to surface(s) of the culture vessel. PASCs do not produce teratomas in vivo, nor do they induce immunorejection upon transplantation, and they achieve a high efficiency in grafting. The cells and compositions can be used for cell therapy and to screen new drugs.
Inventor(s): Chazenbalk; Gregorio (Studio City, CA)
Assignee: THE REGENTS OF THE UNIVERSITY OF CALIFORNIA (Oakland, CA)
Application Number:14/893,014
Patent Claims:1. A method of isolating pluripotent stem cells (PSCs) from adipose tissue, said method comprising: (a) releasing adipose cells, including an adipocyte fraction and a stromal vascular fraction, from an adipose tissue sample using a proteolytic enzyme that breaks the peptide bonds in collagen; (b) co-incubating the released adipocytes and the released stromal vascular fraction for 2-36 hours, wherein 4-24 hours of said co-incubation takes place under stress conditions in a medium containing a proteolytic enzyme, in the absence of nutrients, under hypoxic conditions, and decreasing the temperature to 4.degree. C.; (c) recovering the viable cells following the co-incubation in step (b) by centrifuging to produce a cell pellet, removing supernatant containing adipocyte cell debris by aspiration, washing the cell pellet to remove the proteolytic enzyme, and resuspending the recovered cells in media; and (d) optionally culturing the recovered cells.

2. The method of claim 1, wherein the proteolytic enzyme of step (a) is collagenase.

3. The method of claim 1, wherein the proteolytic enzyme of step (b) is collagenase.

4. The method of claim 1, wherein the method is performed without cell-sorting.

5. The method of claim 1, wherein the adipose tissue sample of step (a) is 50-2000 ml, and wherein the recovering of step (c) comprises recovering at least 1,000,000 pluripotent adipose-derived stem cells (PASCs) within 24 hours of initiating the stress conditions of step (b).

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