Patent Application
20140301989
The discovery of pluripotent cells in adipose tissue has revealed a novel source of cells that may be used for autologous cell therapy to regenerate tissue. These pluripotent cells reside in the “stromal” or “non-adipocyte” fraction of the adipose tissue; they were previously considered to be pre-adipocytes, i.e. adipocyte progenitor cells, however recent data suggest a much wider differentiation potential. Zuk et al. were able to establish differentiation of such subcutaneous human adipose stromal cells (“ASCs”) in vitro into adipocytes, chondrocytes and myocytes. Zuk P A, et al. Mol Biol Cell 13(12):4279-4295, 2002. These findings were extended in a study by Erickson et al., which showed that human ASCs could differentiate in vivo into chondrocytes following transplantation into immune-deficient mice. Erickson G R, el al. Biochem Biophys Res Commun. 2002; 290:763-669. More recently, it was demonstrated that human ASCs were able to differentiate into neuronal cells, osteoblasts cardiomyocyte, and endothelial cells. The key benefit of using pluripotent ASCs for autologous cell therapy is the ease by which they can be isolated and their relative abundance.
In at least one embodiment of a method of cell-based therapy of the present disclosure, the method comprises the steps of exposing at least one mammalian stem cell expressing mesenchymal-epithelial transition factor (c-Met) to a compound operable to phosphorylate c-Met, and administering the at least one mammalian stem cell to a patient, where the patient may have a vascular deficiency. In at least one embodiment, the step of administering the at least one mammalian stem cell treats the patient's vascular deficiency. Further, the at least one mammalian stem cell may originally be isolated from the patient. Optionally, the at least one mammalian stem cell may be isolated from a source selected from the group consisting of adipose tissue, peripheral blood, blood vessels, and umbilical cord blood. The at least one mammalian stem cell in an exemplary embodiment may comprise an adipose stromal cell. Additionally, in at least one embodiment of the method of cell-based therapy of the present disclosure, the compound may be at least one of hepatocyte growth factor (HGF), a fragment of HGF operable to bind to c-Met, a monoclonal antibody specific for c-Met, a c-Met agonist (such as a small molecule or nucleic acid), or a stressing agent, such as one comprising hydrogen peroxide.
In at least one embodiment of a method of cell-based therapy of the present disclosure, the step of exposing the at least one mammalian cell may be for at least one minute, for at least fifteen minutes, or for at least about one hour. Additionally, the step of administering the at least one mammalian stem cell of the present disclosure may comprise intravenously injecting the at least one mammalian stem cell into the patient, where the patient may be a mammal, such as a human. Further, the step of administering may, in at least one embodiment of the present disclosure, cause at least one of a regeneration of at least one tissue of the patient, and/or a relative increase in blood perfusion of an ischemic tissue in the patient.
In at least one embodiment of a method of cell-based therapy of the present disclosure, the method comprises the steps of exposing at least one mammalian stem cell expressing mesenchymal-epithelial transition factor (c-Met) to an environmental condition operable to phosphorylate c-Met, and administering the at least one mammalian stem cell to a patient, wherein the environmental condition may in at least one embodiment be is selected from a group consisting of hypoxia, and serum starvation.
In at least one embodiment of a method of treating a patient of the present disclosure, the method comprises the steps of exposing at least one adipose stromal cell to an effective amount of an agonist for mesenchymal-epithelial transition factor (c-Met), and administering the at least one adipose stromal cell to treat a patient in need. The at least one mammalian stem cell of the present disclosure may be isolated from a source selected from the group consisting of adipose tissue, peripheral blood, blood vessels, and umbilical cord blood. Additionally, the at least one mammalian stem cell may be isolated from the patient. Further, the at least one adipose stromal cell may be capable of regenerating at least one tissue of the patient. Moreover, the step of administering the at least one mammalian cell may cause a relative increase in blood perfusion of an ischemic tissue in the patient.
In at least one embodiment of a method of treating a patient of the present disclosure, the method comprises steps of introducing a nucleotide segment encoding hepatocyte growth factor (HGF) into at least one adipose stromal cell (ASC), and administering the at least ASC to treat a patient in need. Optionally, the step of introducing a nucleotide segment may cause the level of HGF in the at least one adipose stromal cell to increase. The nucleotide segment of an embodiment of the present disclosure may be a viral vector. Additionally, the step of administering the at least ASC of the present disclosure to treat a patient in need may comprise intravenously injecting the at least one mammalian stem cell into the patient, where the patient may be a mammal, such as a human. Further, the step of administering the at least one ASC of the present disclosure causes the regeneration of at least one tissue of the patient, and/or a relative increase in blood perfusion of an ischemic tissue in the patient.
In at least one embodiment of a kit for enhancing the efficacy of ASC cells of the present disclosure, the kit comprises a first container, a composition contained within the first container; wherein the composition comprises HGF, a second container comprising a bolus of ASC, and instructions for treatment of the bolus of ASC with the composition.
The above-mentioned embodiments and other features, advantages and disclosures contained herein, and the manner of attaining them, will become apparent and the present disclosure will be better understood by reference to the following description of various exemplary embodiments of the present disclosure taken in conjunction with the accompanying drawings, wherein:
For the purposes of promoting an understanding of the principles of the present disclosure, reference will now be made to the embodiments illustrated in the drawings, and specific language will be used to describe the same. It will nevertheless be understood that no limitation of the scope of this disclosure is thereby intended.
The disclosure of the present application provides various methods for the alteration of the protein activity of adipose stromal cells (“ASC”). The methods disclosed herein increase the efficacy of ASCs as they relate to therapeutic treatment of patients.
There exists an important need for advancement of cell-based therapies due to mammalian diseases and conditions which are currently untreatable or undertreated with current therapies. Given that the levels of cells required for effective cell-based therapies may not available, or secondary considerations may prohibit the use of large numbers of cells, a need exists for increasing the efficacy and safety of cell-based therapies.
While ASCs secrete many beneficial factors and promote reperfusion and tissue repair in ischemia models, knock-down of hepatocyte growth factor (HGF) by RNA interference (RNAi) attenuates ASC potency in vivo in a murine hindlimb ischemia model. Compared to ASC expressing normal levels of HGF, modified ASC demonstrate reduced persistence in repaired tissues. A series of in vitro and in vivo experiments described herein show that c-Met acts in promoting ASC-mediated repair of ischemic tissues and is part of a previously uncharacterized HGF/c-Met autocrine loop.
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In an exemplary embodiment of the method 100 of cell therapy, the step 104 of administering the at least one mammalian stem cell treats the patient's vascular deficiency. Additionally, the at least one mammalian stem cell may be originally isolated from the patient. The patient may in at least one embodiment may be a non-human or human mammal. Further, the at least one mammalian stem cell may, in at least one embodiment, be isolated from a source selected from the group consisting of adipose tissue, peripheral blood, blood vessels, and umbilical cord blood. Additionally, the at least one mammalian stem cell, in at least one exemplary embodiment, comprises an adipose stromal cell. Further, according to at least one exemplary embodiment, the at least one mammalian stem cell may comprise a mesenchymal cell. The mesenchmal cell may be derived from any available cell type, including, but not limited to, bone marrow, skin, and myocytes.
In an exemplary embodiment of the method 100 of cell therapy, the compound may be hepatocyte growth factor (HGF), a fragment thereof which is operable to bind to c-Met, or a monoclonal antibody specific to c-Met.
In an exemplary embodiment of the method 100 for cell therapy, the step 102 of exposing the at least one mammalian cell may be for at least one minute, fifteen minutes, or one hour. Additionally, the step 104 of administering may comprise intravenously injecting the at least one mammalian stem cell into the patient. Further, the step 104 of administering may cause the regeneration of at least one tissue of the patient and/or the relative increase in blood perfusion of an ischemic tissue in the patient
According to a further exemplary embodiment of the method 100 for cell therapy, the compound may be a c-Met agonist. The c-Met agonist, in at least one embodiment, may be a small molecule or a nucleic acid. Additionally, in an exemplary embodiment, the compound may be a stressing agent. The stressing agent, in at least one embodiment, may comprise hydrogen peroxide.
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In an exemplary embodiment of method 200, the at least one adipose stromal cell is capable of regenerating at least one tissue of the patient, and/or causing a relative increase in blood perfusion of an ischemic tissue in the patient.
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In an exemplary embodiment of treating a patient according to an embodiment of the present disclosure, the at least one adipose stromal cell is capable of regenerating at least one tissue of the patient, and/or causing a relative increase in blood perfusion of an ischemic tissue in the patient. Further, the step of administering the at least one mammalian stem cell into the patient, according to at least one embodiment of the present disclosure, may be through intravenous injection.
According to at least one embodiment of a kit for enhancing the efficacy of ASCs in the treatment of a patient of the present disclosure, the kit comprising a first container, a composition contained within the first container, wherein the composition comprising HGF. In at least this exemplary embodiment, the kit further comprises a second container comprising a bolus of ASC, and instructions for treatment of the bolus of ASC with the composition.
Dual-cassette lentiviral vectors, expressing green fluorescent protein (GFP) and either a small hairpin RNA (shRNA) specific for HGF mRNA (shHGF) or a control sequence (shCtrl), were used to stably transduce ASCs (ASC-shHGF or ASC-shCtrl). Activation of c-Met was blocked by incubating ASC for 1 hr in the presence of 10 p.M of the selective inhibitor PHA-665752 (Pfizer). Hyper-stimulation of c-Met phosphorylation was accomplished by treating for 1 hr with 100ng/ml purified recombinant HGF (R&D Systems). After both treatments, cells were washed with PBS before infusion. Cells were infused by tail vein infusion 24 hr after surgically inducing unilateral hindlimb ischemia in immunocompromised mice (N>6 /group). Reperfusion was monitored by laser Doppler perfusion imaging (Moor Systems). GFP cells were quantitated by fluorescent microscopic imaging of thin sections from the gastrocnemius muscles of ischemic and non-ischemic limbs. Apoptosis of GFP cells was measured in situ with an ApopTag kit (Chemicon). The relative levels of phosphorylated-Akt (p-Akt) and total Akt were determined by Western blotting with antibodies specific to each (Upstate).
The levels of HGF expressed by ASCs are reduced by shRNA. ASC stably transduced with an shRNA targeted to the HGF gene secrete more than 4-fold less HGF into the medium during culture compared to ASC-shCtrl cells (
The pro-survival action of activated c-Met is transduced in part through PI3K/Akt, which plays a critical role in controlling survival and apoptosis. Western blot analysis of total and phosphorylated Akt (pAkt) after subjecting cells to the stress of serum deprivation for twelve hours indicated that the level of pAkt was reduced by 2-fold (p<0.01) in ASC-shHGF cells compared to ASC-shCtrl (
While reduced HGF expression in ASC does not appear to significantly affect the homing of ASCs to the injury site, the reduction in HGF does affect the persistence in injured tissues in vivo. The results of these in vivo experiments showed that there was no difference in total GFP-positive cells in ischemic limbs at 5 days after infusion of 106 ASC, indicating similar homing potentials (
Detection of GFP-labeled shCtrl- and shHGF-ASC in ischemic and non-ischemic muscles was conducted at 1, 5 and 20 days following cell infusion. At the indicated times after cell infusion 3 mice were sacrificed and the gastrocnemius muscles from both limbs were removed and fixed. The entire muscle was sectioned into 10-15 thin sections, each separated by 100-gm intervals. Thin sections (5 gm) were stained with GFP and anti-smooth muscle a-actin antibodies. Sections were also stained with 4′,6-diamidino-2-phenylindole dihydrochloride to visualize nuclei. Images of sections were obtained at 400× magnification. Ten randomly selected images were analyzed with Image J software.
Suppression of HGF increases the frequency of ASC undergoing apoptosis in ischemic but not normal tissues. However, significantly more ASC-shHGF cells were apoptotic than ASC-shCtrl cells (61+0.1% vs. 41%+3.2%, respectively, P<0.01) (
Further, there was no significant difference in apoptosis percentages in normal tissues (13.1±6.8% and 14.9±6.4% for ASC-shCtrl and ASC-shHGF, respectively). By 20 days following infusion, 3-fold fewer ASC-shHGF were present in ischemic tissues compared to ASC-shCtrl (p<0.01) (
ASCs possess a functional HGF/c-Met autocrine loop that is influential in cellular survival in adverse environments. Disruption of this cycle has reduced the ability of ASC to withstand stresses associated with the ischemic environment and, thus, their ability to affect tissue rescue and repair. The link between the HGF/c-Met autocrine loop and survival under adverse conditions was examined directly either by specifically inhibiting c-Met phosphorylation with the selective inhibitor PHA-665752 or, conversely, by stimulating greater phosphorylation with excess HGF (
The efficacy of ASC can be enhanced by HGF pretreatment. Hindlimb ischemia was surgically induced in immunotolerant NS2 mice (N=6/group). At 24 hours after surgery the mice received tail vein injections of saline control or 3×105 untreated ASC or the same number of ASC that had been treated for 1 hour with PHA or HGF (
In addition to the paracrine effects of HGF expression on recovery of host tissues from ischemic insult described above, these results establish that HGF is necessary for autocrine promotion of ASC survival and consequent efficacy. Importantly, we have shown in at least one embodiment that increased survival and potency can be attained with only a brief and reversible treatment immediately before administration.
Treatment of human ASC (h-ASC) under various environmental conditions may increase the level of phosphorylation of c-Met. Exposure of h-ASC to hydrogen peroxide is shown herein to increase the level of phosphorylation of c-Met (See
The methods of modification of ASC of the present disclosure have various benefits to the treatment of patient diseases and conditions. For example, the phosphorylation of c-Met by HGF may increase the efficacy of ASC when used as a therapeutic in a patient.
While various embodiments of methods for the treatment of ASCs, and patients, have been described in considerable detail herein, the embodiments are merely offered by way of non-limiting examples of the disclosure described herein. It will therefore be understood that various changes and modifications may be made, and equivalents may be substituted for elements thereof, without departing from the scope of the disclosure. Indeed, this disclosure is not intended to be exhaustive or to limit the scope of the disclosure.
Further, in describing representative embodiments, the disclosure may have presented a method and/or process as a particular sequence of steps. However, to the extent that the method or process does not rely on the particular order of steps set forth herein, the method or process should not be limited to the particular sequence of steps described. Other sequences of steps may be possible. Therefore, the particular order of the steps disclosed herein should not be construed as limitations of the present disclosure. In addition, disclosure directed to a method and/or process should not be limited to the performance of their steps in the order written. Such sequences may be varied and still remain within the spirit and scope of the present disclosure.
Cal L, Johnstone B H, Cook TG, Liang Z, Traktuev D, Cornetta K, Ingram D A, Rosen E D, March K L, Suppression of hepatocyte growth factor production impairs the ability of adipose stromal cells to promote ischemic tissue revascularization., Stem Cells, 2007, 25(12)3234-43.
The present International Patent Application is related to, and claims the priority benefit of, U.S. Provisional Patent Application Ser. No. 61/498,079, filed on Jun. 17, 2011, the contents of which are hereby incorporated into the present disclosure in their entirety.
This invention was made with government support from the National Institutes of Health under grant number HL 077688. The U.S. Government has certain rights in the present disclosure.
| Filing Document | Filing Date | Country | Kind | 371c Date |
|---|---|---|---|---|
| PCT/US12/42952 | 6/18/2012 | WO | 00 | 12/20/2013 |
| Number | Date | Country | |
|---|---|---|---|
| 61498079 | Jun 2011 | US |
