CA2327631A1 - Inflammatory cytokine secretion inhibition - Google Patents
Inflammatory cytokine secretion inhibition Download PDFInfo
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- CA2327631A1 CA2327631A1 CA002327631A CA2327631A CA2327631A1 CA 2327631 A1 CA2327631 A1 CA 2327631A1 CA 002327631 A CA002327631 A CA 002327631A CA 2327631 A CA2327631 A CA 2327631A CA 2327631 A1 CA2327631 A1 CA 2327631A1
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Abstract
A process of decreasing the expression of one or more of the inflammatory cytokines IFN-.gamma., IL-6 and IL-12 from cells in a mammalian patient, comprises administering to the patient an effective amount of stressed mammalian blood cells, said stressed cells having been extracorporeally subjected to at least one stressor selected from oxidative stress and ultraviolet radiation.
Description
?AOM NIXON VANDEAHYE PC (TUE) 12. 5' 00 12:37/ST. 12:31/N0, 4261594651 P 14 INFLAMMATORY CYTOKINE SECRETION INHIBITION
Field of the Invention This invention relates to treatment of biological cells and immune system modulation. More specifically, it relates to treatment of cells of the mammalian immune system to alter the cytokine profiles of certain types of constituent cells, and therapeutic applications of such treatments.
Background of the Invention The mammalian immune system comprises lymphocytes (one type of white blood cell), the major components of which are B cells, which mature within the bone marrow, and T cells which migrate from the bone marrow to mature in the thymus gland. B cells react to antigens to proliferate and differentiate into memory B cells and effector B cells to generate and express antibodies specific to the antigen, to combat it. T cells have T cell receptors which recognize antigen associated with MHC molecules on a cell, to differentiate into memory T cells and various types of effector T cells- The T cell population is made up of T-helper (TH) cells and T-cytotoxic (T~) cells, distinguished from one another by the presence of surface membrane glycoprotein CD4 on TH cells and surface membrane glycoprotein CD8 on TC cells. Activation of a TH cell can cause it to secrete various growth factors (cytokines). Different types of TH cells secrete different cytokines.
These cytokines play key roles in the immune response, including autoimmune responses.
One type of TH cell, known as T,.,1, expresses cytokines which, in excessive amounts, can cause inflammation in the mammalian body. Examples of such inflammatory cytokines include interferon~y (IFN-y), interleukin-6 (iL-6) and interleukin-12 (IL-12). When the body produces inappropriately large amounts of inflammatory cytokines, significantly more than endogenous levels found in the corresponding non-diseased tissue of healthy individuals, either through over-activation of TH1 Cells, activation of excessive numbers of TH1 cells, or a switch of ~~ Z
TOM NIXON VANDERHYE PC (TUE) 12. 5' 00 12:38/ST. 12:31/N0. 4261594651 f ! 5 other types of T cells to the TH1 type to create excessive numbers of cytokines expressing TH1 cells, an inflammatory disorder can manifest itself in a patient.
Summary of the Invention The present invention provides a process whereby expression of inflammatory cytokines including IFN-y, IL-6 and IL.-12, either individually or in combination, is reduced in a mammalian patient body. The process involves introducing into the patient blood cells which have been extracorporeally stressed by subjection to an oxidative stress and/or ultraviolet radiation. On introduction of these stressed blood cells, there is a reduction the expression of one or more of these inflammatory cytokines, either by down regulating TN1 cells, or perhaps by decreasing the population of TH1 cells, e.g. by causing a switch of T cells from TH1 to TH2. Whatever the precise mechanism of action, the result is a significant and measurable decrease in these inflammatory cytokines in the patient's system.
Accordingly, the process of the invention is useful in the medical treatment of patients suffering from, prone to or at risk of contracting a disorder associated with excessive amounts of one or more of the inflammatory cytokines lFNry, Il.-6 and !L-12 (e.g. chronic fatigue syndrome - ses Cannon et.al., "Acute phase responses and cytokine secretion in chronic fatigue syndrome", J.Clin. lmmunol. 1999 Nov:
19(6): 414-21; and Gupta, S. et.al., Int. J. MoLMed.. 1999 Feb; 3(2): 209-13).
Thus according to the present invention, there is provided a process of decreasing the expression of one or more of the inflammatory cytokines IFNry, IL-6 and IL-12 from cells in a mammalian patient, which comprises administering to the patient an effective amount of stressed mammalian blood cells, said stressed cells having been extracorporeally subjected to at least one stressor selected from oxidative stress and ultraviolet radiation.
There is further provided a method for treating an inflammatory disease condition in a patient mediated by inflammatory cytokine production, which method comprises administering to the patient an effective amount of 30M NIXON. VANDEAHYE PC (TUE) 12. 5' 00 12:38/ST. 12:31/N0, 4261594651 P 16 _3_ stressed mammalian blood cells wherein said stressed mammalian blood cells have been extracorporeally subjected to at least one stressor selected from oxidative conditions and ultraviolet radiation.
Brief Reference to the Drawings The accompanying Figures 1 and 2 are graphical presentations of the results of the experiment reported below as a specific Example.
Description of the Preferred Embodiments A preferred embodiment of the invention is a process of decreasing the expression of !L-6 and IL-12 from cells in a mammalian patient, which comprises administering to the patient an effective amount of stressed mammalian blood cells, said stressed cells having been extracorporeally subjected to at least one stressor selected from oxidative stress and ultraviolet radiation. Such a process is useful in treating medical disorders associated with excess expressions or excess presence of cytokine (L-6 and/or cytokine IL-72. A preferred application of the process of the present invention is in the treatment of disorders other than graft versus host disease, and other than autoimmune diseases such as rheumatoid arthritis, psoriasis, scleroderma, lupus, diabetes mellitus, organ rejection, miscarriage, multiple sclerosis, inflammatory bowel disease and atherosclerosis, and other than contact hypersensitivity disorders.
A particularly preferred embodiment is a process of decreasing 1L-6 expression from cells in a mammalian patient which comprises administering to the patient an effective amount of stressed mammalian blood cells, said stressed cells having been extracorporeally subjected to at least one stressor selected from oxidative stress and ultraviolet radiation. This process is particularly useful in alleviation of disorders such as chronic fatigue syndrome.
The source of the stressed blood cells for use in the present invention is preferably the patient's own blood, i.e. an aliquot of autologvus blood.
t?0~ NIXON VANDEAHYE PC (TUE) 12, 5' 00 12:40/ST. 12:31/N0. 4261594651 F 17 The terms 'aliquot' ; ' aliquot of blood.' or similar terms used herein include whole blood, separated cellular fractions of the blood including platelets, separated non-cellular fractions of the blood including plasma, plasma components and combinations thereof. Preferably, in human patients, the volume of the aliquot is up to about 400 ml, preferably from about 0.1 to about 100 ml, more preferably from about 7 to about 15 ml, even more preferably from about 8 to about 72 ml, and most preferably about 10 ml. The effect of the stressor or the combination of stressors is to modify the blood, and/or the cellular or non-cellular fractions thereof, contained in the aliquot. The modified aliquot is then re-introduced into the subjects body by any suitable method, most preferably intrarnuscular injection, but also including subcutaneous injection, intraperitoneal injection, intra-arterial injection, intravenous injection and oral administration, following which it causes decrease in the expression of one or more of the inflammatory cytokines INF-~, IL-6 and IL-72.
According to a preferred process of the present invention, an aliquot of blood is extracted from a mammalian subject, preferably a human, and the aliquot of blood is treated ex vivo. simultaneously or sequentially, with the aforementioned stressors. Then it is injected back into the same subject.
Preferably a combination of both of the aforementioned stressors is used.
Preferably also, the aliquot of blood is in addition subjected to mechanical stress. Such mechanical stress is suitably that applied to the aliquot of blood by extraction of the blood aliquot through a conventional blood extraction needle, or a substantially equivalent mechanical stress, applied shortly before the other chosen stressors are applied to the blood aliquot. This mechanical stress may be supplemented by the mechanical stress exerted on the blood aliquot by bubbling gases through it, such as ozone/vxygen mixtures, as described below.
Optionally also, a temperature stressor may be applied to the blood aliquot, simultaneously or sequentially with the other stressors, i.e. a temperature at, above or below body temperature.
AON NIXON VANDERHYE PC 1TUE) 12. 5' 00 12:40/ST. 12;31/N0. 4261594651 P 18 The optionally applied temperature stressor either warms the aliquot being treated to a temperature above normal body temperature or cools the aliquot below normal body temperature. The temperature is selected so that the temperature stressor does not cause excessive hemolysis in the blood contained in the aliquot, and so that, when the treated aliquot is injected into a subject, the desired effect will be achieved, without development of significant adverse side effects_ Preferably, the temperature stressor is applied so that the temperature of all or a part of the aliquot is up to about 55°C, and more preferably in the range of from about -5°C to about 55°C.
In some preferred embodiments of the invention, the temperature of the aliquot is raised above normal body temperature, such that the mean temperature of the aliquot does not exceed a temperature of about 55°C, more preferably from about 40°C to about 50°C, even more preferably from about 40°C
to about 44°C, and most preferably about 42.5 ~ 1 °C.
(n other preferred embodiments, the aliquot is cooled below normal body temperature such that the mean temperature of the aliquot is within the range of from about 4°C to about 36.5°C, more preferably from about 10°C to about 30°C, and even more preferably from about 15°C to about 25°C.
The oxidative environment stressor can be the application to the aliquot of solid, liquid or gaseous oxidizing agents. Preferably, it involves exposing the aliquot to a mixture of medical grade oxygen and ozone gas, most preferably by applying to the aliquot medical grade oxygen gas having ozone as a component therein. The ozone content of the gas stream and the flow rate of the gas stream are preferably selected such that the amount of ozone introduced to the blood aliquot, either on its own or in combination with one of the other stressors, does not give rise to excessive levels of cell damage , without significant adverse side effects.
,.
Suitably, the gas stream has an ",_;Y,1 CA 02327631 2000-12-05 ROM NIXON VANDERHYE PC (TUE112. 5'00 12:41/ST,12:31/N0,4261594651 P 19 ozone content of up to about 300 ~.g/ml, preferably up to about 7 00 ~,g/ml, more preferably about 30 ~.g/ml, even mere preferably up to about 20 ~,g/ml, particularly preferably from about 10 ~g/ml to about 20 ~g/ml, and most preferably about 14.5 f 1.0w g/ml. The gas stream is suitably supplied to the aliquot at a rate of up to about 2.0 litres/rnin, preferably up to about 0.5 litres/min, more preferably up to about 0.4 litres/min, even more preferably up to about 0.33 litres/min, and most preferably about 0.24 ~ 0.024 litres/min. The lower limit of the flow rate of the gas stream is preferably not lower than O.Oi litres/min, more preferably not lower than 0.1 litres/min, and even more preferably not lower than 0.2 litres/min , all rates at STP.
The ultraviolet light stressor is suitably applied by irradiating the aliquot under treatment from a source of UV light. Preferred UV sources are UV
lamps emitting UV-C band wavelengths, i.e. at wavelengths shorter than about nm. Ultraviolet light corresponding to standard UV-A (wavelengths from about to about 400 nm) and UV-B (wavelengths from about 280 to about 315) sources can also be used. As in the case of the oxidative stressor, the UV dose should be selected, on its own or in combination of the other chosen stressor(s), so that excessive amounts of cell damage do not occur, and so that, when the treated aliquot is injected into a subject, the desired effect will be achieved. For example, an appropriate dosage of such UV light, can be obtained from up to eight lamps arranged to be exposed to the sample container holding the aliquot, operated at an intensity to deliver a total UV light energy at 253.7 nm at the surface of the blood of from about 0.025 to about 10 jvules/cm2, preferably from about 0.1 to about 3.0 joules/cm2. Such a treatment, applied in combination with the oxidative environment stressor, provides a modified blood aliquot which is ready for injection into the subject.
It is preferred to subject the aliquot to the oxidative environment stressvr, the UV light stressor and the temperature stressor simultaneously, following the subjection of the aliquot to the mechanical stress, e.g. by extraction of the blood from the patient. Thus, the aliquot may be maintained at a predetermined temperature above or below body temperature while the =ROM NIXON VANDERHYE PC (TUE) 12. 5' 00 12:41/ST. 12:31/N0, 4261594651 P 2~~
oxygen/ozone gas mixture is applied thereto and while it is irradiated with ultraviolet light.
The time for which the aliquot is subjected to the stressors is normally within the time range of from about 0.5 minutes up to about 60 minutes.
The time depends to some extent upon the chosen combination of stressors.
When UV light is used, the intensity of the UV light rnay affect the preferred time.
The chosen temperature level may also affect the preferred time. When oxidative environment in the form of a gaseous mixture of oxygen and ozone applied to the aliquot is chosen as one of the two stressors, the concentration of the oxidizing agent and the rate at which it is supplied to the aliquot may affect the preferred temperature. Some routine experimentation to establish optimum times may be necessary on the part of the operator, once the other stressor levels have been set, such experimentation being well within the skill of the art. Under most stressor conditions, preferred times will be in the approximate range of from about 2 to about 5 minutes, more preferably about 3 minutes. The starting blood temperature, and the rate at which it can be warmed or cooled to a predetermined temperature, tends to vary from subject to subject. Warming is suitably by use of one or more infrared lamps placed adjacent to the aliquot container. Other methods of warming can also be adopted.
As noted, it is preferred to subject the aliquot of blood to a mechanical stressor, as well as the chosen stressor(s) discussed above.
Extraction of the blood aliquot from the patient through an injection needle constitutes the most convenient way of obtaining the aliquot for further extracorporeal treatment, and this extraction procedure imparts a suitable mechanical stress to the blood aliquot. The mechanical stressor may be supplemented by subsequent processing, for example the additional mechanical shear stress caused by bubbling as the oxidative stressor is applied.
In the practice of the preferred process of the present invention, the blood aliquot may be treated with the heat, UV light and oxidative environment =ROM NIXON VANDERHYE PC (TUE)12. 5'00 12:41/ST.12:31/N0.4261594551 P 21 _g_ stressors using an apparatus of the type described in aforementioned U.S.
Patent No. 4,968,483 to Mueller. The aliquot is placed in a suitable, sterile container, which is fitted into the machine. A UV-permeable container is used and the UV
lamps are switched on for a fixed period before the other stressor is applied, to allow the output of the UV lamps to stabilize. When a temperature stressor is used combination, the UV lamps are typically on while the temperature of the aliquot is adjusted to the predetermined preferred value, s.g. 42.5 f 1 °C. Four UV lamps are suitably used, placed around the container.
(n the preferred method of the invention, a mammalian patient under treatment for an IFN-~y mediated disorder, an 1L-6 mediated disorder and/or a mediated disorder is given one or more courses of treatments, each course of treatment comprising the administration to a mammalian subject of one or more (e.g. one to six or one to twelve) aliquots of mammalian blood modified as discussed above.
For optimum effectiveness of the treatment, it is preferred that no more than one aliquot of modified blood be administered to the subject per day, in one or more injection sites, and that the maximum rest period between any two consecutive aliquots during the course of treatment be no greater than about
Field of the Invention This invention relates to treatment of biological cells and immune system modulation. More specifically, it relates to treatment of cells of the mammalian immune system to alter the cytokine profiles of certain types of constituent cells, and therapeutic applications of such treatments.
Background of the Invention The mammalian immune system comprises lymphocytes (one type of white blood cell), the major components of which are B cells, which mature within the bone marrow, and T cells which migrate from the bone marrow to mature in the thymus gland. B cells react to antigens to proliferate and differentiate into memory B cells and effector B cells to generate and express antibodies specific to the antigen, to combat it. T cells have T cell receptors which recognize antigen associated with MHC molecules on a cell, to differentiate into memory T cells and various types of effector T cells- The T cell population is made up of T-helper (TH) cells and T-cytotoxic (T~) cells, distinguished from one another by the presence of surface membrane glycoprotein CD4 on TH cells and surface membrane glycoprotein CD8 on TC cells. Activation of a TH cell can cause it to secrete various growth factors (cytokines). Different types of TH cells secrete different cytokines.
These cytokines play key roles in the immune response, including autoimmune responses.
One type of TH cell, known as T,.,1, expresses cytokines which, in excessive amounts, can cause inflammation in the mammalian body. Examples of such inflammatory cytokines include interferon~y (IFN-y), interleukin-6 (iL-6) and interleukin-12 (IL-12). When the body produces inappropriately large amounts of inflammatory cytokines, significantly more than endogenous levels found in the corresponding non-diseased tissue of healthy individuals, either through over-activation of TH1 Cells, activation of excessive numbers of TH1 cells, or a switch of ~~ Z
TOM NIXON VANDERHYE PC (TUE) 12. 5' 00 12:38/ST. 12:31/N0. 4261594651 f ! 5 other types of T cells to the TH1 type to create excessive numbers of cytokines expressing TH1 cells, an inflammatory disorder can manifest itself in a patient.
Summary of the Invention The present invention provides a process whereby expression of inflammatory cytokines including IFN-y, IL-6 and IL.-12, either individually or in combination, is reduced in a mammalian patient body. The process involves introducing into the patient blood cells which have been extracorporeally stressed by subjection to an oxidative stress and/or ultraviolet radiation. On introduction of these stressed blood cells, there is a reduction the expression of one or more of these inflammatory cytokines, either by down regulating TN1 cells, or perhaps by decreasing the population of TH1 cells, e.g. by causing a switch of T cells from TH1 to TH2. Whatever the precise mechanism of action, the result is a significant and measurable decrease in these inflammatory cytokines in the patient's system.
Accordingly, the process of the invention is useful in the medical treatment of patients suffering from, prone to or at risk of contracting a disorder associated with excessive amounts of one or more of the inflammatory cytokines lFNry, Il.-6 and !L-12 (e.g. chronic fatigue syndrome - ses Cannon et.al., "Acute phase responses and cytokine secretion in chronic fatigue syndrome", J.Clin. lmmunol. 1999 Nov:
19(6): 414-21; and Gupta, S. et.al., Int. J. MoLMed.. 1999 Feb; 3(2): 209-13).
Thus according to the present invention, there is provided a process of decreasing the expression of one or more of the inflammatory cytokines IFNry, IL-6 and IL-12 from cells in a mammalian patient, which comprises administering to the patient an effective amount of stressed mammalian blood cells, said stressed cells having been extracorporeally subjected to at least one stressor selected from oxidative stress and ultraviolet radiation.
There is further provided a method for treating an inflammatory disease condition in a patient mediated by inflammatory cytokine production, which method comprises administering to the patient an effective amount of 30M NIXON. VANDEAHYE PC (TUE) 12. 5' 00 12:38/ST. 12:31/N0, 4261594651 P 16 _3_ stressed mammalian blood cells wherein said stressed mammalian blood cells have been extracorporeally subjected to at least one stressor selected from oxidative conditions and ultraviolet radiation.
Brief Reference to the Drawings The accompanying Figures 1 and 2 are graphical presentations of the results of the experiment reported below as a specific Example.
Description of the Preferred Embodiments A preferred embodiment of the invention is a process of decreasing the expression of !L-6 and IL-12 from cells in a mammalian patient, which comprises administering to the patient an effective amount of stressed mammalian blood cells, said stressed cells having been extracorporeally subjected to at least one stressor selected from oxidative stress and ultraviolet radiation. Such a process is useful in treating medical disorders associated with excess expressions or excess presence of cytokine (L-6 and/or cytokine IL-72. A preferred application of the process of the present invention is in the treatment of disorders other than graft versus host disease, and other than autoimmune diseases such as rheumatoid arthritis, psoriasis, scleroderma, lupus, diabetes mellitus, organ rejection, miscarriage, multiple sclerosis, inflammatory bowel disease and atherosclerosis, and other than contact hypersensitivity disorders.
A particularly preferred embodiment is a process of decreasing 1L-6 expression from cells in a mammalian patient which comprises administering to the patient an effective amount of stressed mammalian blood cells, said stressed cells having been extracorporeally subjected to at least one stressor selected from oxidative stress and ultraviolet radiation. This process is particularly useful in alleviation of disorders such as chronic fatigue syndrome.
The source of the stressed blood cells for use in the present invention is preferably the patient's own blood, i.e. an aliquot of autologvus blood.
t?0~ NIXON VANDEAHYE PC (TUE) 12, 5' 00 12:40/ST. 12:31/N0. 4261594651 F 17 The terms 'aliquot' ; ' aliquot of blood.' or similar terms used herein include whole blood, separated cellular fractions of the blood including platelets, separated non-cellular fractions of the blood including plasma, plasma components and combinations thereof. Preferably, in human patients, the volume of the aliquot is up to about 400 ml, preferably from about 0.1 to about 100 ml, more preferably from about 7 to about 15 ml, even more preferably from about 8 to about 72 ml, and most preferably about 10 ml. The effect of the stressor or the combination of stressors is to modify the blood, and/or the cellular or non-cellular fractions thereof, contained in the aliquot. The modified aliquot is then re-introduced into the subjects body by any suitable method, most preferably intrarnuscular injection, but also including subcutaneous injection, intraperitoneal injection, intra-arterial injection, intravenous injection and oral administration, following which it causes decrease in the expression of one or more of the inflammatory cytokines INF-~, IL-6 and IL-72.
According to a preferred process of the present invention, an aliquot of blood is extracted from a mammalian subject, preferably a human, and the aliquot of blood is treated ex vivo. simultaneously or sequentially, with the aforementioned stressors. Then it is injected back into the same subject.
Preferably a combination of both of the aforementioned stressors is used.
Preferably also, the aliquot of blood is in addition subjected to mechanical stress. Such mechanical stress is suitably that applied to the aliquot of blood by extraction of the blood aliquot through a conventional blood extraction needle, or a substantially equivalent mechanical stress, applied shortly before the other chosen stressors are applied to the blood aliquot. This mechanical stress may be supplemented by the mechanical stress exerted on the blood aliquot by bubbling gases through it, such as ozone/vxygen mixtures, as described below.
Optionally also, a temperature stressor may be applied to the blood aliquot, simultaneously or sequentially with the other stressors, i.e. a temperature at, above or below body temperature.
AON NIXON VANDERHYE PC 1TUE) 12. 5' 00 12:40/ST. 12;31/N0. 4261594651 P 18 The optionally applied temperature stressor either warms the aliquot being treated to a temperature above normal body temperature or cools the aliquot below normal body temperature. The temperature is selected so that the temperature stressor does not cause excessive hemolysis in the blood contained in the aliquot, and so that, when the treated aliquot is injected into a subject, the desired effect will be achieved, without development of significant adverse side effects_ Preferably, the temperature stressor is applied so that the temperature of all or a part of the aliquot is up to about 55°C, and more preferably in the range of from about -5°C to about 55°C.
In some preferred embodiments of the invention, the temperature of the aliquot is raised above normal body temperature, such that the mean temperature of the aliquot does not exceed a temperature of about 55°C, more preferably from about 40°C to about 50°C, even more preferably from about 40°C
to about 44°C, and most preferably about 42.5 ~ 1 °C.
(n other preferred embodiments, the aliquot is cooled below normal body temperature such that the mean temperature of the aliquot is within the range of from about 4°C to about 36.5°C, more preferably from about 10°C to about 30°C, and even more preferably from about 15°C to about 25°C.
The oxidative environment stressor can be the application to the aliquot of solid, liquid or gaseous oxidizing agents. Preferably, it involves exposing the aliquot to a mixture of medical grade oxygen and ozone gas, most preferably by applying to the aliquot medical grade oxygen gas having ozone as a component therein. The ozone content of the gas stream and the flow rate of the gas stream are preferably selected such that the amount of ozone introduced to the blood aliquot, either on its own or in combination with one of the other stressors, does not give rise to excessive levels of cell damage , without significant adverse side effects.
,.
Suitably, the gas stream has an ",_;Y,1 CA 02327631 2000-12-05 ROM NIXON VANDERHYE PC (TUE112. 5'00 12:41/ST,12:31/N0,4261594651 P 19 ozone content of up to about 300 ~.g/ml, preferably up to about 7 00 ~,g/ml, more preferably about 30 ~.g/ml, even mere preferably up to about 20 ~,g/ml, particularly preferably from about 10 ~g/ml to about 20 ~g/ml, and most preferably about 14.5 f 1.0w g/ml. The gas stream is suitably supplied to the aliquot at a rate of up to about 2.0 litres/rnin, preferably up to about 0.5 litres/min, more preferably up to about 0.4 litres/min, even more preferably up to about 0.33 litres/min, and most preferably about 0.24 ~ 0.024 litres/min. The lower limit of the flow rate of the gas stream is preferably not lower than O.Oi litres/min, more preferably not lower than 0.1 litres/min, and even more preferably not lower than 0.2 litres/min , all rates at STP.
The ultraviolet light stressor is suitably applied by irradiating the aliquot under treatment from a source of UV light. Preferred UV sources are UV
lamps emitting UV-C band wavelengths, i.e. at wavelengths shorter than about nm. Ultraviolet light corresponding to standard UV-A (wavelengths from about to about 400 nm) and UV-B (wavelengths from about 280 to about 315) sources can also be used. As in the case of the oxidative stressor, the UV dose should be selected, on its own or in combination of the other chosen stressor(s), so that excessive amounts of cell damage do not occur, and so that, when the treated aliquot is injected into a subject, the desired effect will be achieved. For example, an appropriate dosage of such UV light, can be obtained from up to eight lamps arranged to be exposed to the sample container holding the aliquot, operated at an intensity to deliver a total UV light energy at 253.7 nm at the surface of the blood of from about 0.025 to about 10 jvules/cm2, preferably from about 0.1 to about 3.0 joules/cm2. Such a treatment, applied in combination with the oxidative environment stressor, provides a modified blood aliquot which is ready for injection into the subject.
It is preferred to subject the aliquot to the oxidative environment stressvr, the UV light stressor and the temperature stressor simultaneously, following the subjection of the aliquot to the mechanical stress, e.g. by extraction of the blood from the patient. Thus, the aliquot may be maintained at a predetermined temperature above or below body temperature while the =ROM NIXON VANDERHYE PC (TUE) 12. 5' 00 12:41/ST. 12:31/N0, 4261594651 P 2~~
oxygen/ozone gas mixture is applied thereto and while it is irradiated with ultraviolet light.
The time for which the aliquot is subjected to the stressors is normally within the time range of from about 0.5 minutes up to about 60 minutes.
The time depends to some extent upon the chosen combination of stressors.
When UV light is used, the intensity of the UV light rnay affect the preferred time.
The chosen temperature level may also affect the preferred time. When oxidative environment in the form of a gaseous mixture of oxygen and ozone applied to the aliquot is chosen as one of the two stressors, the concentration of the oxidizing agent and the rate at which it is supplied to the aliquot may affect the preferred temperature. Some routine experimentation to establish optimum times may be necessary on the part of the operator, once the other stressor levels have been set, such experimentation being well within the skill of the art. Under most stressor conditions, preferred times will be in the approximate range of from about 2 to about 5 minutes, more preferably about 3 minutes. The starting blood temperature, and the rate at which it can be warmed or cooled to a predetermined temperature, tends to vary from subject to subject. Warming is suitably by use of one or more infrared lamps placed adjacent to the aliquot container. Other methods of warming can also be adopted.
As noted, it is preferred to subject the aliquot of blood to a mechanical stressor, as well as the chosen stressor(s) discussed above.
Extraction of the blood aliquot from the patient through an injection needle constitutes the most convenient way of obtaining the aliquot for further extracorporeal treatment, and this extraction procedure imparts a suitable mechanical stress to the blood aliquot. The mechanical stressor may be supplemented by subsequent processing, for example the additional mechanical shear stress caused by bubbling as the oxidative stressor is applied.
In the practice of the preferred process of the present invention, the blood aliquot may be treated with the heat, UV light and oxidative environment =ROM NIXON VANDERHYE PC (TUE)12. 5'00 12:41/ST.12:31/N0.4261594551 P 21 _g_ stressors using an apparatus of the type described in aforementioned U.S.
Patent No. 4,968,483 to Mueller. The aliquot is placed in a suitable, sterile container, which is fitted into the machine. A UV-permeable container is used and the UV
lamps are switched on for a fixed period before the other stressor is applied, to allow the output of the UV lamps to stabilize. When a temperature stressor is used combination, the UV lamps are typically on while the temperature of the aliquot is adjusted to the predetermined preferred value, s.g. 42.5 f 1 °C. Four UV lamps are suitably used, placed around the container.
(n the preferred method of the invention, a mammalian patient under treatment for an IFN-~y mediated disorder, an 1L-6 mediated disorder and/or a mediated disorder is given one or more courses of treatments, each course of treatment comprising the administration to a mammalian subject of one or more (e.g. one to six or one to twelve) aliquots of mammalian blood modified as discussed above.
For optimum effectiveness of the treatment, it is preferred that no more than one aliquot of modified blood be administered to the subject per day, in one or more injection sites, and that the maximum rest period between any two consecutive aliquots during the course of treatment be no greater than about
2~
days. As used herein, the term "rest period" is defined as the number of days between consecutive aliquots or consecutive courses of treatment on which no aliquots of modified blood are administered to the subject.
Therefore, except where aliquots are administered to the subject on consecutive days, a rest period of from 1 to 21 days is provided between any two aliquots during the course of treatment. Moreover, at least one of the rest periods during the course of treatment preferably has a length of about 3 to 15 days.
Although it may be sufficient to administer only one course of treatment as described above to the subject, it may be preferred in some circumstances to administer more than one course of treatment, or to follow the sOM NIXON VANDERHYE PC (TUE) 12. 5' 00 12:42/ST, 12:31/N0, 4261594651 P 22 _9-above-described course of treatment by periodic "booster" treatments, if necessary, to maintain the desired effects of the present invention. For example, it may be preferred to administer booster treatments at intervals of 3 to 4 months following the initial course of treatment, or to administer a second course of treatments to the subject following a rest period of several weeks or months.
The invention is further illustrated and described with reference to the fouowing specific example, comprising animal studies conducted in an approved manner.
EXAMPLE
As a measure of the effect of the process of the present invention on inflammation resulting from T cell secretions, a contact hypersensitivity (CHS) test was used, according to approved animal experimentation procedures, using the method described by Kondo et, al., "Lymphocyte function associated antigen-1 (LFA-1 ) is required for maximum elicitation of allergic contact dematitis" Br J.Dermatol. 131:354-359, 1994, with minor variations.. The disclosure thereof is incorporated herein by reference. Briefly, to induce CNS, the abdominal skin of each mouse was shaved and painted with dinitrodifluorobenzene DNFB, the sensitizing chemical, using 25 ~I of 0.5% DNFB in 4:1 acetone:olive oil solution.
This sensitization was applied to four groups of five Balb/c mice. In addition, a measure of the responsible cytokines was made.
Whole blood was obtained from Baib/c mice, by extraction from a main artery through an injection needle, and treated with an anti-coagulant.
An aliquot of this was subjected to the process described herein, to obtain treated blood. The remainder was left untreated, for use in control experiments. Since these mice are genetically identical, the administration of the treated blood to others of the group is equivalent to administration of the treated blood to the donor animal.
70N NIXON VANDEAHYE PC (TUE) 12. 5' 00 12:42/ST. 12:31/N0. 4261594651 P
To obtain treated blood, the selected aliquot, in a sterile, UV-transmissive container, was treated simultaneously with a gaseous oxygen/ozone mixture and ultraviolet light at elevated temperature using an apparatus as generally described in aforementioned U.S. Patent No. 4,968,483 Mueller et.al.
Specifically, 12 ml of citrated blood was transferred to a sterile, low density polyethylene vessel (more specifically, a Vasogen vC7oo2 Blood container) for ex vIVO treatment with stressors according to the invenlivn. Using an apparatus as described in the aforementioned Mueller patent (more specifically, a Vasogen VC7oo~ apparatus), the blood was heated to 42.511 °C and at that temperature irradiated with UV light principally at a wavelength of 253.7 nm, while oxygeNozone gas mixture was bubbled through the blood to provide the oxidative environment and to facilitate exposure of the blood to UV. The constitution of the gas mixture was 14.5 t 1.0 ~g ozone/ml, with the remainder of the mixture comprising medical grade oxygen. The gas mixture was bubbled through the aliquot at a rate of 240 ~ 24 ml/min for a period of 3 minutes.
Of the 4 groups of sensitized mice, the first, control group A-7 received n4 treatment. The second, control group B-1, was treated with physiological saline, 50Ee1. The third, control group C-1, was sham treated, with 501.d of blood which had been extracted but not treated with the stressors. The fourth, test group D-1, was treated with 501 of blood subjected to stressors as described above_ Treatments, each involving intramuscular injection of 50 111 of the respective liquid, started on the day of sensitization, and was repeated every day for a total of 6 days. On the same day as the last treatment, but after its administration, the animals were challenged with DNFB, by applying to the ears of each animal l0t~l of 0.2% solution of DNFB. Inflammation due to CHS manifests itself in a swelling of the ears. Ear thickness was measured, 24 hours after challenge, with a Peacock spring-loaded micrometer (Ozaki Co., Tokyo, Japan). The results were expressed as the change (from pre-challenge level) in ear thickness and represent the mean maximal increase at 24 hours after challenge.
Lymph nodes were drained from each of the animals after the AOM NIXON VANDERHYE PC (TUE)12. 5'00 12:43/ST,12:31/N0,4261594651 P 24 conclusion of the above procedures, and the lymph tissue tested, by standard, known rtPCR technology, for expression of the mRNA of the cytokines IFN-y, IL-and IL-12. This process of testing and analysis followed the procedures described in Kondo, S., et.al., (1996) J.Immunology, p.157;4822. Thus the PCR products were determined by scanning of photonegatives using a laser densitometer, and the densitometric value of the IFN~y was normalized tv that of the housekeeping gene B-actin. The analyses indicated that animals which had received a course of injection of blood subjected to stressors as described had significantly reduced IFN-y, IL-6 and IL-12 as compared with sham treated animals and controls, as illustrated in the accompanying Figures, in general correlation with the anti-inflammation results.
days. As used herein, the term "rest period" is defined as the number of days between consecutive aliquots or consecutive courses of treatment on which no aliquots of modified blood are administered to the subject.
Therefore, except where aliquots are administered to the subject on consecutive days, a rest period of from 1 to 21 days is provided between any two aliquots during the course of treatment. Moreover, at least one of the rest periods during the course of treatment preferably has a length of about 3 to 15 days.
Although it may be sufficient to administer only one course of treatment as described above to the subject, it may be preferred in some circumstances to administer more than one course of treatment, or to follow the sOM NIXON VANDERHYE PC (TUE) 12. 5' 00 12:42/ST, 12:31/N0, 4261594651 P 22 _9-above-described course of treatment by periodic "booster" treatments, if necessary, to maintain the desired effects of the present invention. For example, it may be preferred to administer booster treatments at intervals of 3 to 4 months following the initial course of treatment, or to administer a second course of treatments to the subject following a rest period of several weeks or months.
The invention is further illustrated and described with reference to the fouowing specific example, comprising animal studies conducted in an approved manner.
EXAMPLE
As a measure of the effect of the process of the present invention on inflammation resulting from T cell secretions, a contact hypersensitivity (CHS) test was used, according to approved animal experimentation procedures, using the method described by Kondo et, al., "Lymphocyte function associated antigen-1 (LFA-1 ) is required for maximum elicitation of allergic contact dematitis" Br J.Dermatol. 131:354-359, 1994, with minor variations.. The disclosure thereof is incorporated herein by reference. Briefly, to induce CNS, the abdominal skin of each mouse was shaved and painted with dinitrodifluorobenzene DNFB, the sensitizing chemical, using 25 ~I of 0.5% DNFB in 4:1 acetone:olive oil solution.
This sensitization was applied to four groups of five Balb/c mice. In addition, a measure of the responsible cytokines was made.
Whole blood was obtained from Baib/c mice, by extraction from a main artery through an injection needle, and treated with an anti-coagulant.
An aliquot of this was subjected to the process described herein, to obtain treated blood. The remainder was left untreated, for use in control experiments. Since these mice are genetically identical, the administration of the treated blood to others of the group is equivalent to administration of the treated blood to the donor animal.
70N NIXON VANDEAHYE PC (TUE) 12. 5' 00 12:42/ST. 12:31/N0. 4261594651 P
To obtain treated blood, the selected aliquot, in a sterile, UV-transmissive container, was treated simultaneously with a gaseous oxygen/ozone mixture and ultraviolet light at elevated temperature using an apparatus as generally described in aforementioned U.S. Patent No. 4,968,483 Mueller et.al.
Specifically, 12 ml of citrated blood was transferred to a sterile, low density polyethylene vessel (more specifically, a Vasogen vC7oo2 Blood container) for ex vIVO treatment with stressors according to the invenlivn. Using an apparatus as described in the aforementioned Mueller patent (more specifically, a Vasogen VC7oo~ apparatus), the blood was heated to 42.511 °C and at that temperature irradiated with UV light principally at a wavelength of 253.7 nm, while oxygeNozone gas mixture was bubbled through the blood to provide the oxidative environment and to facilitate exposure of the blood to UV. The constitution of the gas mixture was 14.5 t 1.0 ~g ozone/ml, with the remainder of the mixture comprising medical grade oxygen. The gas mixture was bubbled through the aliquot at a rate of 240 ~ 24 ml/min for a period of 3 minutes.
Of the 4 groups of sensitized mice, the first, control group A-7 received n4 treatment. The second, control group B-1, was treated with physiological saline, 50Ee1. The third, control group C-1, was sham treated, with 501.d of blood which had been extracted but not treated with the stressors. The fourth, test group D-1, was treated with 501 of blood subjected to stressors as described above_ Treatments, each involving intramuscular injection of 50 111 of the respective liquid, started on the day of sensitization, and was repeated every day for a total of 6 days. On the same day as the last treatment, but after its administration, the animals were challenged with DNFB, by applying to the ears of each animal l0t~l of 0.2% solution of DNFB. Inflammation due to CHS manifests itself in a swelling of the ears. Ear thickness was measured, 24 hours after challenge, with a Peacock spring-loaded micrometer (Ozaki Co., Tokyo, Japan). The results were expressed as the change (from pre-challenge level) in ear thickness and represent the mean maximal increase at 24 hours after challenge.
Lymph nodes were drained from each of the animals after the AOM NIXON VANDERHYE PC (TUE)12. 5'00 12:43/ST,12:31/N0,4261594651 P 24 conclusion of the above procedures, and the lymph tissue tested, by standard, known rtPCR technology, for expression of the mRNA of the cytokines IFN-y, IL-and IL-12. This process of testing and analysis followed the procedures described in Kondo, S., et.al., (1996) J.Immunology, p.157;4822. Thus the PCR products were determined by scanning of photonegatives using a laser densitometer, and the densitometric value of the IFN~y was normalized tv that of the housekeeping gene B-actin. The analyses indicated that animals which had received a course of injection of blood subjected to stressors as described had significantly reduced IFN-y, IL-6 and IL-12 as compared with sham treated animals and controls, as illustrated in the accompanying Figures, in general correlation with the anti-inflammation results.
Claims
Priority Applications (6)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CA002327631A CA2327631A1 (en) | 2000-12-05 | 2000-12-05 | Inflammatory cytokine secretion inhibition |
| US10/002,634 US20020090360A1 (en) | 2000-12-05 | 2001-12-05 | Inflammatory cytokine secretion inhibition |
| EP20010999376 EP1365842A2 (en) | 2000-12-05 | 2001-12-05 | Inflammatory cytokine secretion inhibition |
| PCT/CA2001/001745 WO2002045723A2 (en) | 2000-12-05 | 2001-12-05 | Inflammatory cytokine secretion inhibition with modified mammalian blood |
| CA002430937A CA2430937A1 (en) | 2000-12-05 | 2001-12-05 | Inflammatory cytokine secretion inhibition |
| AU2002215735A AU2002215735A1 (en) | 2000-12-05 | 2001-12-05 | Inflammatory cytokine secretion inhibition with modified mammalian blood |
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CA002327631A CA2327631A1 (en) | 2000-12-05 | 2000-12-05 | Inflammatory cytokine secretion inhibition |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA2327631A1 true CA2327631A1 (en) | 2002-06-05 |
Family
ID=4167833
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002327631A Abandoned CA2327631A1 (en) | 2000-12-05 | 2000-12-05 | Inflammatory cytokine secretion inhibition |
Country Status (4)
| Country | Link |
|---|---|
| EP (1) | EP1365842A2 (en) |
| AU (1) | AU2002215735A1 (en) |
| CA (1) | CA2327631A1 (en) |
| WO (1) | WO2002045723A2 (en) |
Families Citing this family (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| EP1773360A4 (en) * | 2004-07-20 | 2009-09-02 | Vasogen Ireland Ltd | Acute inflammatory condition treatment |
Family Cites Families (5)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US5980954A (en) * | 1992-02-07 | 1999-11-09 | Vasogen Ireland Limited | Treatment of autoimmune diseases |
| CA2296997A1 (en) * | 2000-01-18 | 2001-07-18 | Vasogen Ireland Limited | Treatment of congestive heart failure |
| CA2297448A1 (en) * | 2000-01-28 | 2001-07-28 | Vasogen Inc. | Improved inhibition of graft versus host disease |
| CA2308105A1 (en) * | 2000-05-11 | 2001-11-11 | Vasogen Ireland Limited | Treatment of il-10 deficiencies |
| CA2309518A1 (en) * | 2000-05-25 | 2001-11-25 | Vasogen Ireland Limited | Apoptotic entities for use in treatment of t-cell-mediated and inflammatory disorders |
-
2000
- 2000-12-05 CA CA002327631A patent/CA2327631A1/en not_active Abandoned
-
2001
- 2001-12-05 AU AU2002215735A patent/AU2002215735A1/en not_active Abandoned
- 2001-12-05 WO PCT/CA2001/001745 patent/WO2002045723A2/en not_active Application Discontinuation
- 2001-12-05 EP EP20010999376 patent/EP1365842A2/en not_active Withdrawn
Also Published As
| Publication number | Publication date |
|---|---|
| EP1365842A2 (en) | 2003-12-03 |
| WO2002045723A2 (en) | 2002-06-13 |
| AU2002215735A1 (en) | 2002-06-18 |
| WO2002045723A3 (en) | 2003-09-04 |
| WO2002045723A9 (en) | 2002-12-19 |
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