TREA

System, method, and composition for removing uremic toxins in dialysis processes

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Information

  • Patent Grant
  • 10980931
  • Patent Number
    10,980,931
  • Date Filed
    Thursday, February 7, 2019
    5 years ago
  • Date Issued
    Tuesday, April 20, 2021
    3 years ago
Information
Abstract
Methods and devices for providing dialysis treatment are provided. The device comprises a cartridge for providing regenerative dialysis, the cartridge comprising: a body having an inlet and an outlet and defining an interior, the interior including at least a layer comprising urease, a layer comprising zirconium oxide, a layer comprising zirconium phosphate, and a layer comprising carbon, wherein at least two of the layers are blended together to provide a gradient of the two materials.
Description
BACKGROUND

The present invention relates generally to methods of treatment. More specifically, the present invention relates to dialysis processes.


Due to disease or insult or other causes, the renal system can fail. In renal failure of any cause, there are several physiological derangements. The balance of water, minerals (Na, K, Cl, Ca, P, Mg, SO4) and the excretion of daily metabolic load of fixed hydrogen ions is no longer possible in renal failure. During renal failure, toxic end products of nitrogen metabolism (urea, creatinine, uric acid, and others) can accumulate in blood and tissues.


Dialysis processes have been devised for the separation of elements in a solution by diffusion across a semi-permeable membrane (diffusive solute transport) down a concentration gradient. Principally, dialysis comprises two methods: hemodialysis and peritoneal dialysis.


Hemodialysis treatment utilizes the patient's blood to remove waste, toxins, and excess water from the patient. The patient is connected to a hemodialysis machine and the patient's blood is pumped through the machine. Catheters are inserted into the patient's veins and arteries to connect the blood flow to and from the hemodialysis machine. Waste, toxins, and excess water are removed from the patient's blood and the blood is infused back into the patient. Hemodialysis treatments last several hours and are generally performed in a treatment center about three or four times per week.


Peritoneal dialysis utilizes a dialysis solution and dialysate, which is infused into a patient's peritoneal cavity. The dialysate contacts the patient's peritoneal membrane in the peritoneal cavity. Waste, toxins, and excess water pass from the patient's bloodstream through the peritoneal membrane and into the dialysate. The transfer of waste, toxins, and water from the bloodstream into the dialysate occurs due to diffusion and osmosis. The spent dialysate is drained from the patient's peritoneal cavity to remove the waste, toxins, and water from the patient.


There are various types of peritoneal dialysis, including continuous ambulatory peritoneal dialysis (CAPD) and automated peritoneal dialysis (APD). CAPD is a manual dialysis treatment in which the patient connects an implanted catheter to a drain and allows a spent dialysate fluid to drain from the peritoneal cavity. The patient then connects to a bag of fresh dialysate and manually infuses the fresh dialysate through the catheter and into the patient's peritoneal cavity. The patient disconnects the catheter from the fresh dialysate bag and allows the dialysate to dwell within the cavity to transfer waste, toxins, and excess water from the patient's bloodstream to the dialysate solution. After the dwell period, the patient repeats the manual dialysis procedure.


In CAPD the patient performs several drain, fill, and dwell cycles during the day, for example, about four times per day. Each treatment cycle typically takes about 3-4 hours. Manual peritoneal dialysis performed by the patient requires a great deal of time and effort by the patient. The patient is routinely inconvenienced leaving ample opportunity for therapy enhancements to improve patient quality of life.


Automated peritoneal dialysis is similar to continuous peritoneal dialysis in that the dialysis treatment includes a drain, fill, and dwell cycle. However, a dialysis machine automatically performs 3-4 cycles of peritoneal dialysis treatment, typically overnight while the patient sleeps.


To this end, a dialysis machine is fluidly connected to an implanted catheter. The dialysis machine is also fluidly connected to a source of fresh dialysate, such as a bag of dialysate solution, and to a fluid drain. The dialysis machine pumps spent dialysate from the peritoneal cavity though the catheter to the drain. Then, the dialysis machine pumps fresh dialysate from the dialysate source through the catheter and into the patient's peritoneal cavity. The dialysis machine allows the dialysate to dwell within the cavity to transfer waste, toxins, and excess water from the patient's bloodstream to the dialysate solution. The dialysis machine is computer controlled so that the dialysis treatment occurs automatically when the patient is connected to the dialysis machine, for example, overnight.


Several drain, fill, and dwell cycles will occur during the treatment. Also, a last fill is typically used at the end of the automated dialysis treatment so that the patient can disconnect from the dialysis machine and continue daily functions while dialysate remains in the peritoneal cavity. Automated peritoneal dialysis frees the patient from manually performing the drain, dwell, and fill steps, and can improve the patient's dialysis treatment and quality of life.


In view of recent developments and therapies, the line between traditional peritoneal dialysis and hemodialysis has become blurred. For example, some therapies use components of both therapies.


A recent therapy is regenerative dialysis. In this system a dialysis system is used that includes a cartridge for dialysate regeneration. The cartridge includes a resin bed including zirconium-based resins. An example of a cartridge that is used in such a system is manufactured under the name Redy by Sorb Technology, Oklahoma City, Okla. This system, however, requires the constant attention of medical personnel. Moreover, the dialysate that is regenerated by the cartridge has an undesirable sodium and pH level. In this regard, the dialysis solution does not have a physiologic pH or electrolyte content. This is especially a problem if the dialysis solution is to be reinfused into the peritoneal cavity of a patient.


SUMMARY

The present invention provides improved systems as well as methods for providing dialysis to a patient. More specifically, in an embodiment, the present invention provides systems, cartridges, and methods for regenerative dialysis therapies. However, it should be noted that the cartridge of the present invention can be used in a variety of therapies including hemodialysis and peritoneal dialysis therapies as well as acute dialysis.


To this end, in an embodiment, a device for removing uremic toxins in a dialysis procedure is provided comprising a body having an inlet and an outlet and defining an interior, the interior including a layer comprising urease, a layer comprising zirconium oxide, a layer comprising zirconium phosphate, and a layer comprising carbon, and the device being so constructed and arranged so that a fluid entering the device contacts the zirconium oxide layer upon entering the device before contacting the urease or the zirconium phosphate layer.


In an embodiment, the zirconium oxide is in bicarbonate form.


In an embodiment, the zirconium oxide is in hydroxyl form.


In an embodiment, the carbon layer is located in juxtaposition to the outlet.


In an embodiment, the fluid flows through a layer of zirconium oxide before entering the carbon layer.


In an embodiment, the zirconium phosphate has a pH of approximately 2 to about 8.


In an embodiment, the zirconium oxide has a pH of approximately 6 to about 13.


In an embodiment, two separate layers of zirconium phosphate are provided.


In an embodiment, two separate layers of zirconium oxide are provided.


In an embodiment, open headers at each of the inlet and outlet end of the device are provided.


In an embodiment, an opening for venting a gas to the atmosphere located at the outlet end is provided.


In an embodiment the urease layer is the first layer.


In an embodiment the zirconium phosphate layer is located before the zirconium oxide layer.


In a further embodiment of the present invention, a cartridge for use in a dialysis system for removing toxins is provided comprising a body having an inlet end and an outlet end. The body includes an interior including at least four layers, the layers including a first layer of a resin selected from the group consisting of zirconium phosphate having a pH of approximately 2.5 to about 5 and urease, a second layer of a resin selected from the group consisting of zirconium oxide having a pH of approximately 9 to about 13 and urease, a third layer of zirconium phosphate, and a fourth layer of zirconium oxide having a pH of approximately 6.5 to about 7.5. The interior is so constructed and arranged that a fluid entering the interior from the first inlet end flows through the first layer, then the second layer, then the third layer, and then the fourth layer.


In an embodiment, the first layer comprises approximately 200 to about 800 grams of zirconium phosphate.


In an embodiment, the fourth layer comprises approximately 50 to about 200 grams of carbon.


In an embodiment, the urease is a cross-linked enzyme.


In yet another embodiment, a device for regenerating a dialysis solution is provided. The device includes a body including a resin bed. The resin bed includes at least a layer of urease, zirconium phosphate, zirconium oxide, and carbon and being so constructed and arranged that a dialysis solution having a pH that is either basic or acidic will exit the cartridge after it passes through the resin bed at a pH of approximately 7 to about 7.8.


In an embodiment, the first layer of the resin bed that the solution contacts is selected from the group consisting of zirconium phosphate having a pH of approximately 2.0 to about 5 and urease.


In an embodiment, the second layer that the solution passes through in the resin bed is selected from the group consisting of zirconium oxide having a pH of approximately 9 to about 13 and urease.


In an embodiment, the third layer of the resin bed that the solution passes through is zirconium phosphate.


In an embodiment, the fourth layer of the cartridge that the solution passes through is zirconium oxide having a pH of approximately 6.8 to about 7.5.


In an embodiment, the pH of the solution exiting the cartridge is approximately 7.4.


In a further embodiment, a device for use in a system for treating a patient with a dialysis solution is provided. The device including an inlet in fluid communication with a source of dialysis solution, a body including the inlet and defining an interior and having an outlet, and the body including a resin bed including a layer of urease, a layer of zirconium oxide, and a layer of zirconium phosphate that define a three layer structure. The resin bed is oriented so that the first layer that the dialysis solution contacts of the three layer structure is either the urease or the zirconium phosphate layer and the zirconium oxide layer is so constructed and arranged that a basic or an acidic dialysis solution entering the inlet will exit the outlet with a physiologically acceptable pH.


In an embodiment, the device is used in a regenerative dialysis system.


Still further, in an embodiment, a method for constructing a cartridge for use in a system for providing dialysis is provided. The method comprising the steps of providing a resin bed including zirconium oxide and zirconium phosphate and selecting and orienting the zirconium oxide and zirconium phosphate to allow the cartridge to remove uremic toxins present in a dialysis solution entering the resin bed and causing the dialysis solution exiting the cartridge to be at a physiological pH and include a physiological electrolyte balance.


In an embodiment, the method includes the steps of providing a body having an inlet and an outlet and defining an interior, the interior including a layer comprising urease, a layer comprising zirconium oxide, a layer comprising zirconium phosphate, and a layer comprising carbon; and the device being so constructed and arranged so that a fluid entering the device contacts the zirconium phosphate layer upon entering the device before contacting the urease on the zirconium oxide layer.


In a yet further embodiment, a method for providing dialysis is provided comprising the steps of removing uremic toxins by passing a dialysis fluid through a body having an inlet and an outlet and defining an interior, the interior including at least four layers, a first layer comprising either zirconium phosphate having a pH of approximately 2.5 to about 5 or urease, a second layer comprising either zirconium oxide having a pH of approximately 9 to about 13 or urease, a third layer comprising zirconium phosphate and a fourth layer comprising zirconium oxide having a pH of approximately 6.8 to about 7.5.


Additionally, in an embodiment, a method of providing regenerative dialysis is provided comprising the step of removing uremic toxins by passing a dialysis fluid through a body having an inlet and an outlet and defining an interior, the interior including at least four layers, a first layer comprising either zirconium phosphate having a pH of approximately 2.5 to about 5 or urease, a second layer comprising either zirconium oxide having a pH of approximately 9 to about 13 or urease, a third layer comprising zirconium phosphate and a fourth layer comprising zirconium oxide having a pH of approximately 6.8 to about 7.5.


An advantage of the present invention is to provide an improved dialysis procedure.


Moreover, an advantage of the present invention is to provide an improved cartridge for removing impurities from a dialysis fluid.


Still, an advantage of the present invention is to provide an improved system for providing dialysis.


Further, an advantage of the present invention is to provide an improved cartridge that can be used in a single loop or multiple loop system.


Additionally, an advantage of the present invention is to provide an improved resin bed for a cartridge for a dialysis system.


Additionally, an advantage of the present invention is to provide an improved cartridge that is constructed and arranged so that dialysis solution that exits the cartridge has a physiological pH and electrolyte content.


Additional features and advantages are described herein, and will be apparent from, the following Detailed Description and the figures.





BRIEF DESCRIPTION OF THE FIGURES


FIG. 1 illustrates schematically a system for performing dialysis pursuant to the present invention.



FIG. 2 illustrates a cross-sectional view of an embodiment of the cartridge of the present invention.



FIG. 3 illustrates graphically ammonium effluent concentration (ppm) versus mass ammonium delivered (mEq) for zirconium phosphate available from two suppliers (Sorb technologies and magnesium elektron).



FIG. 4 illustrates graphically sodium capacity as a function of zirconium oxide pH.



FIG. 5 illustrates an embodiment of a cross-sectional view of a resin bed of a cartridge of the present invention.



FIG. 6 illustrates a further embodiment of a resin bed of a cartridge of the present invention.



FIG. 7 illustrates a still further embodiment of a resin bed of a cartridge of the present invention.



FIGS. 8-10 illustrate graphically the results of Experiment No. 2.



FIG. 11 illustrates the system that was used in Experiment No. 3 for testing the cartridges of the present invention.



FIGS. 12a-c illustrates a cross-sectional view of the layers of the cartridge used in Experiment No. 3.



FIGS. 13a-c illustrate pH, sodium bicarbonate profiles of samples taken pursuant to Experiment No. 3.



FIGS. 14a-d represent pH, sodium and bicarbonate profiles and urea conversion of samples taken pursuant to Experiment No. 3.



FIGS. 15a-c illustrate pH, bicarbonate and sodium profiles of samples over time pursuant to Experiment No. 3.



FIG. 15d illustrates the urea conversion over time pursuant to Experiment No. 3.





DETAILED DESCRIPTION

The present invention relates to methods of providing dialysis treatment. Additionally, the present invention relates to systems for providing dialysis. More specifically, in an embodiment, the present invention provides improved cartridges that are used to remove uremic toxins.


In a preferred embodiment, the present invention relates to systems and components for use in continuous flow peritoneal dialysis procedure. However, it should be noted that the present invention can be used in a variety of methods for providing dialysis including hemodialysis and peritoneal dialysis


Continuous flow peritoneal dialysis is achieved by continuously infusing into and draining from the peritoneum a solution. For example, a closed loop or recirculating dialysis can be used where the solution is continuously recirculated to the patient. This can have the advantage of substantially reducing the amount of solution needed for a treatment. However, it is necessary to regenerate the solution with the exact glucose and electrolyte requirements required by the patient. This therapy is designed to be performed primarily at night.


Generally, the system comprises a disposable set including a pump cassette, cartridge, dialyzer, and solution concentrate. FIG. 1 illustrates generally a schematic of the system 10 for providing dialysis treatment pursuant to the present invention.


As illustrated in FIG. 1, two loops are provided: a patient loop 11; and a regeneration loop 12. However, it should be noted that the present invention can be used in a system including only one loop or more than two loops. The patient loop 11 is used to dialyze the patient 14 with dialysate. The regeneration loop 12 is used to regenerate the dialysate. As illustrated generally, the dialysate is pumped from a bag 16 in the patient loop 11 into the patient 14 through a catheter 24. Spent fluid is then fed from the patient 14 back into the dialyzer 20.


A variety of components can be used in the patient loop. In a preferred embodiment a dual lumen catheter 24 is used. The dual lumen catheter provides for continuous, flow in to and out of the peritoneal cavity of the patient. To this end, the dual lumen catheter is implanted in the patient. An example of a catheter for use in the system 10 of the present invention is disclosed in U.S. patent application Ser. No. 09/689,508, filed on Oct. 12, 2000, and entitled “Peritoneal Dialysis Catheter,” the disclosure of which is incorporated herein by reference. However, it should be noted that two single lumen catheters can be used as well as a single lumen catheter.


To regenerate the dialysate, the regeneration loop 12 is provided. In the embodiment illustrated, the regeneration loop 12 preferably includes concentrate in a container 26, a cartridge 32, an ultrafiltrate (UF) pump, and a UF collection means that communicates with the patient loop 11 via the dialyzer 20. A concentrate pump is provided to pump the concentrate 26 from the container through fluid path 27. The fluid in the regeneration loop is pumped through the dialyzer 20 in a counter current fashion to the fluid in the patient loop 11.


The dialyzer 20 is provided to remove water and small solutes such as urea, and creatinine from spent dialysate in the patient loop 11. The dialyzer 20 provides a sterile independent barrier between the patient loop 11 and the regeneration loop 12. Any dialyzer 20 can be used that provides a high clearance of small molecules across the dialyzer. Uric acid will diffuse across the dialyzer, ultrafiltrate is also removed.


It should be noted that although the cartridge 32 of the present invention is illustrated as being used in a two loop system, it can be used in other systems. For example, it is envisioned that the cartridge can be used in a one loop system.


Referring now to FIG. 2, a cross-sectional view of an embodiment of the cartridge 32 of the present invention is illustrated. The cartridge 32 includes a resin bed 34 that is designed to modify the chemistry of the recirculating dialysate and remove uremic toxins. At the same time, pursuant to the present invention, the cartridge 32 maintains electrolyte concentrations and the solution pH of the dialysate at physiologic levels.


The cartridge 32 generally comprises: a main body 40, an inlet cap 42, the resin bed 34, and an outlet cap 44. In the embodiment illustrated, fluid is routed into the cartridge 32 through the inlet cap 42 that is located at a bottom 46 of the cartridge 32. In the embodiment illustrated, a small open header chamber 48 prior to the resin bed 34 is used to distribute the flow of fluid evenly across the cross-section of the cartridge 32 and thereby the resin bed 34. The fluid preferably flows upwardly through the resin bed 34.


In the embodiment illustrated, downstream of the final section of the resin bed 34 there is located another open header chamber 50. The second open header chamber 50 is located before a gas separation chamber 52. The second header chamber 50 is used to maintain an even fluid velocity distribution throughout the resin bed 34.


The liquid level in the gas separation chamber 52 is maintained within a specified range to provide an air space above the liquid in the cartridge 32. Gases that are produced during therapy, e.g., carbon dioxide, are vented from the cartridge 32 to the environment through a passage 54 on the outlet cap 44. If desired, this passage 54 may include a filter member. A submerged, or partially submerged, barrier in the gas separation chamber 52 produces a flow pattern that restricts gases from being drawn to the liquid outlet.


At the outlet cap 44 of the cartridge 32 the liquid outlet port 58 is located. The liquid outlet 58 port removes liquid from the chamber of the cartridge 32 through the outlet cap 44 using a siphon action. If desired, an additional port may be used to add a chemical concentrate to the volume of liquid in the gas separation chamber to reconstitute the chemical composition of the fluid outflow.


In an embodiment, the interior of the cartridge 32 has a rough surface. The rough surface is designed so that it prevents fluid from flowing along the sides of the exterior by passing the resin bed 34.


The resin bed 34, in part, functions to remove waste. In this regard, generally waste is removed using a two-step process. The steps consist of an enzymatic conversion of urea using urease followed by subsequent removal of the conversion byproducts. In the enzymatic reaction, one mole of urea is decomposed into two moles of ammonia and one mole of carbon dioxide. Ammonia (NH3) is primarily (>95%) present as ammonium ion (NH4+), since its pH of 9.3 is substantially greater than the solution pH. The carbon dioxide that is formed can either be present as dissolved carbon dioxide or as bicarbonate ion, depending on the solution pH. Since the pH for this equilibrium is 6.1, both species may be present in substantial quantities under conditions of use. In addition, if the solution is in communication with a gas phase, the dissolved carbon dioxide is in equilibrium with the carbon dioxide present in the gas phase.


The resin bed includes at least four layers, although more layers can be used. Generally, the layers of the resin bed comprise at least: a urease layer; a layer of zirconium phosphate; a layer of zirconium oxide; and a layer of carbon.


The purpose of the urease layer is to enzymatically convert urea that is present in the solution that is flowing through the resin bed 34 to ammonia and carbon dioxide. In solution, ammonia acts as a base since the formation of ammonium results from the donation of H+. Similarly carbon dioxide (CO2) acts as an acid, since the formation of bicarbonate (HCO3) donates H+ to solution. The net result of the urease reaction is to increase the pH.


In an embodiment, 25 to 250 mg of urease are used, although any amount of urease can be used that is sufficient to convert the urea present in the solution to ammonia and carbon dioxide. Preferably, urease comprises the first or second layer of the resin bed.


A variety of urease materials can be used. For example, crosslinked enzyme crystals of urease (Urease-CLEC) can be used. This material is ultra pure and has high specific activity. Therefore, a very small quantity of this urease is sufficient to provide the desired urea-conversions.


By way of example, the amount of urease-CLEC required was optimized for two different internal diameters of the cartridge, 3¼″ and 1¼″ respectively. Next, in order to determine the optimal contact time between urease-CLEC and the substrate stream, the enzyme was blended with powdered Zirconium Oxide (ZO). Table 1 shows the optimized amount of urease-CLEC and ZO required to obtain a urea conversion >90%. The quantity of enzyme used was stable to sterilization with 40 kGy γ-radiation. The flow rate used in all above experiments was 100 ml/min.









TABLE 1







Summary of urease-CLEC required for urea conversion











Column
Amount of

γ-



Diameter
urease-CLEC
Amount of ZO
sterilization
% Urea


(inch)
required (mg)
required (gm)
dose (kGy)
Conversion














1.25
50
25
>40
90


3.25
150
150
>40
97









For this particular approach of using urease-CLEC, the primary challenge is in the development of procedures for blending very small quantities of urease-CLEC with large quantities of ZO. Where as, the small quantity is advantageous for easy containment within the polymer matrix of an ultrafiltration membrane. The use of these urease-impregnated ultrafiltration membranes provide several benefits over the currently available methods:


1) Better urease containment.


2) Reduced cartridge size resulting in enhanced ease of use by patient.


3) Ease of use during cartridge manufacture


4) Increased safety over the existing system (due to better containment of urease in the cartridge)


Table 2 shows the urea conversion observed at various flow rates using a urease-CLEC impregnated membrane. The membrane tested had a diameter of 1 inch, thus, the flow rates used were 1.3, 2.7 and 5.3 ml/min, which correspond to a flux of 50, 100 and 200 ml/min through a 3.25 inch membrane.









TABLE 2







Sample results obtained from a γ-sterilized


urease-CLEC-impregnated membrane











Amount of


γ-



Urease-CLEC
Membrane
Flow rate
sterilization
% Urea


(mg)
diameter (inch)
(ml/min)
dose (kGy)
Conversion














15.85
1
1.3
40
87.3


15.85
1
2.7
40
79.2


15.85
1
5.3
40
66.9









Although, the urea conversions observed are lower than required, better conversions can be expected from membranes prepared with larger quantities of urease-CLEC. Additionally by employing two membranes in each cartridge a higher overall urea conversion can be obtained.


By way of further example, alumina-stabilized urease can also be used. Upon wetting, the urease dissolves but, it is immediately absorbed by the alumina particles that are located in close proximity. The end result is urease that is physically absorbed by the alumina in close proximity. This urease exposed to γ-irradiation at a dose of 15 kGy in the presence of γ-irradiation retained 75% of its initial activity.


Referring now to the zirconium phosphate layer, zirconium phosphate can absorb, under certain conditions, ammonium ion, calcium, magnesium, and sodium. Ammonium ion is removed from solution via an ion exchange process using zirconium phosphate. Zirconium phosphate contains two counter-ions—hydrogen (H) and sodium (Na+). Release of the counter-ions is determined by the solution pH and the current loading state of the resin. In addition to its role as an ion exchange resin, zirconium phosphate also has a considerable buffering capacity.


If the loading state pH of the resin is 6.2 then when in contact with an (acidic) solution having a pH of less than 6.2, the resin will release Na+ in exchange for H+, even in the absence of any other ions. In contact with a (basic) solution having a pH of greater than 6.2, the resin will release H+ in exchange for Na+, even in the presence of other cations. In contact with a solution having a pH of 6.2 and containing ammonium, the resin will exchange a mixture of Na+ and H+ ions for NH4+ such that its equilibrated pH remains unchanged. The zirconium phosphate resin possesses excellent capacity for ammonium, and this capacity is unaffected by changes in equilibrated pH within a given range (pH 6.0-7.2).


The desired pH of the zirconium phosphate will depend, in part, on its location in the resin bed, e.g., the component it is designed to remove. To this end, the zirconium phosphate layer can have a pH of between approximately 2 to about 8. Preferably, zirconium phosphate is present in a range of approximately 200 to about 800 grams. The amount of zirconium phosphate necessary is at a minimum that amount that is sufficient to remove the ammonium that is generated. The level of ammonium generated is determined by the urea that is to be removed by the cartridge. Thus, the amount of zirconium phosphate equals the ammonium to be removed divided by the capacity of the zirconium phosphate, to remove ammonium, which can be determined experimentally.


For example, a process for determining the quantity of zirconium phosphate required in the device can be determined as follows. Equilibrium data is employed to make a first pass guess at the amount of zirconium phosphate required. For a given cartridge containing a particular amount of zirconium phosphate, the effluent ammonium concentration profile is obtained. The capacity of a given cartridge is defined as the mass of ammonium delivered at the time that the effluent concentration exceeds a prescribed level. In an embodiment, this effluent cutoff level is set at 20 ppm. For example, in the data from FIG. 3, for a small prototype device, the ammonium capacity is approximately 4.2 mEq for 10.5 g zirconium phosphate, an input concentration of 3.9 mEq/L ammonium, and a bulk flow rate of 8.3 mL/min (breakthrough at the 20 ppm level occurs after absorption of 4.2 mEq ammonium).


In an embodiment, it is believed that the quantity of zirconium phosphate required is on the order of approximately 600 to about 800 g. In an embodiment, zirconium phosphate will comprise more than half of the cartridge by weight. As to its location in the resin bed, preferably zirconium phosphate can comprise the first layer through all but the last layer of the resin bed (not including the carbon layer). Moreover, multiple zirconium phosphate layers can be used.


Referring now to the zirconium oxide layer, zirconium oxide resin is an amphoteric resin. This means that the resin's ion exchange properties are dependent on the solution pH. If the solution pH is much lower than the pH of the resin, the resin acts as an anion exchange resin. If the solution pH is much greater than the pH of the resin, the resin acts as a cation exchange resin. If the solution pH is near its pH, the resin demonstrates properties of a mixed bed, exchanging both cations and anions. This latter behavior of a mixed bed occurs throughout the physiologic pH range.


The zirconium oxide layer removes phosphates. The zirconium oxide layer, depending on the pH, can also function to remove sodium. Preferably the zirconium oxide layer has a pH of approximately 6 to about 13.


The phosphate capacity of the resin is very high, thus, the size of the layer is governed by how much sodium needs to be removed. In like fashion, the amount of zirconium oxide is thereby determined by the capacity of the zirconium oxide that is used to remove sodium. FIG. 4 illustrates graphically the sodium capacity of zirconium oxide as a function of its pH.


The zirconium oxide layer functions to remove any phosphate that may not have been absorbed by the other components of the resin bed. Further, the zirconium oxide layer controls the pH of the solution leaving the cartridge. Accordingly, preferably the zirconium oxide layer, if it is the last layer (not including the carbon layer) of the cartridge 32, has a pH of approximately 7 to about 9 and in a preferred embodiment, approximately 7.4. Although preferably the zirconium oxide layer is the last layer (not including the carbon layer), multiple zirconium oxide layers can be used.


In an embodiment, zirconium oxide is utilized that has been modified by removing the nitrate ion as the counter ion. In this regard, the nitrate ion was exchanged with bicarbonate ion by treating the zirconium oxide with 15% sodium carbonate solution to a pH of approximately 11.3. The mixture was then washed extensively with water to remove residue sodium nitrate and sodium carbonate. The resin was then dried under high vacuum at an RT of approximately 24 hours. The resulting resin (0.5 g/mL in water) at a pH of approximately 8.5, and a conductivity of 155.1 us/cm. The dried resin was further modified by suspending the resin in water and adding hydrochloric acid until a pH of 7 was achieved. Following the pH adjustment, the resin was washed to remove residual chloride and sodium ions. After each of the washing steps the resin filtrate pH and conductivity was measured. After wash 1, the paper pH was 6.5 to 7 and conductivity 464 us/cm; after wash 2, paper pH 6.5 to 7 and conductivity 186.5 us/cm; and wash 3 pH (paper) 6.5 to 7, conductivity 38.2 us/cm. It should be noted that washes 1 and 2 were performed by letting the mixture settle and then decanting the supernatant to waste. After wash 3, the solid was collected via vacuum filtration through a 0.2 micron pore size nylon filter. The solid was dried via vacuum on the filter apparatus between 6 to 12 hours to yield the final product.


Referring now to the carbon layer, carbon removes creatinine, uric acid or other organic molecules that still may be present in the solution. For example, the carbon layer removes creatinine. The amount of creatinine that needs to be removed by this cartridge is approximately 0.5 g to about 3.0 g. Although the volume of carbon can comprise a wide range, preferably approximately 50 to about 200 grams of carbon is used. Preferably, the carbon will be of the type that has the ability to remove less than 30 grams of glucose from the peritoneal dialysis solution. Thus, such a carbon layer will not remove an excess amount of glucose from the dialysis solution. Activated carbon sold under the designation LP-50 by Carbochem, Ardmore, Pa., has been found to function satisfactorily in this regard. Other carbons can be used. It is believed that carbons that are coconut shell based having a particle size of 20×50 will also work. It should be noted that the carbon layer can be located as any of the layers in the resin bed, although in a preferred embodiment it is the last layer.



FIG. 5 illustrates an embodiment of the resin bed 34 of the present invention. The resin bed 34, in the illustrated embodiment includes five layers 60, 62, 63, 64, and 66. The first layer 60 is a zirconium phosphate layer having a pH of approximately 2.5 to about 5 and comprising approximately 160 grams. The second layer 62 is a layer of urease comprising approximately 25-250 mg of urease-CLEC in 25 gm zirconium phosphate/zirconium oxide or 50-100 gm of urease which is not crosslinked from other sources. The third layer 63 comprises zirconium phosphate having a pH of approximately 7 to about 7.5; preferably there are approximately 380 grams of zirconium phosphate. The fourth layer 64 is approximately 50 to about 75 grams of zirconium oxide at a pH of approximately 5 to about 7.5. The last layer 66 comprises approximately 50 to about 200 grams of carbon and in an embodiment, 130 grams.


In the resin bed 34 the first layer 60 is used to remove sodium, Ca, and Mg. Also this layer 60 will adjust the pH of the solution facilitating the conversion of urea to ammonium by the urease, second layer 62. The third layer 63 removes the ammonium generated by the urease layer 62. To this end, the zirconium phosphate needs to have a pH of greater than or equal to 5; in the illustrated embodiment the pH is 7 to 7.5. The fourth layer 64 of zirconium oxide removes the phosphate and adjusts the pH to approximately 7.4. The size of the fourth layer 64 needs to be such so as to allow the pH of the solution that exists the resin bed 34 to be adjusted to the desired pH. The last layer 66 is the carbon layer that removes any remaining impurities including creatinine.


In CFPD it is required to remove anywhere from approximately 5 to about 20 gm urea/day. Table 1 below provides the amount of resin required for the various layers in order to remove 5, 10, and 20 gm of urea.


For example, removal of 10 gm of urea generates 342 mmol of ammonia and 171 mmol of bicarbonate. Using the resin bed of FIG. 4 to remove 342 mmol of ammonia, a 380 gm layer of zirconium phosphate (resin pH=6.2, ammonia capacity=0.9 mmol/gm resin) was found to be necessary. In the process of removing the 342 mmol of ammonia the resin will release 342 mmol of sodium into the solution. Zirconium phosphate at pH of 6.2 has a capacity of 0.63 mmol/gm resin for sodium and hence will re-adsorb 342-127 mmol of sodium. As a result, an additional 127 mmol of sodium needs to be removed from the solution after passing through layer 63. Layer 60, which is also made up of zirconium phosphate removes this amount of sodium. The amount of zirconium phosphate required to remove this amount of sodium varies as a function of pH of the resin. Table 3 shows the amount of zirconium phosphate at various pHs required to remove 127 mmol of sodium. The amount of zirconium phosphate at various pHs required to remove sodium is equal to:


sodium capacity (mmol/gm resin)=7.1-1.945 (pH of ZP) and 0.138 (pH of Zp)2.


Accordingly, at a pH of 2.5, the sodium capacity is 3.1 mmol/gm ZP. From Table 3, at a pH of 7.2, to remove 171 mmol of sodium we need 53.4 gm of zirconium phosphate.


The size of the zirconium oxide layer is controlled by the amount required to raise the pH from 6.2 to neutral during the entire therapy time. This amount is easily obtained from the pH profile curve. A gram of zirconium oxide resin has the capacity to raise the pH of approximately 0.45 L of solution from 6.2 to neutral. In an embodiment of a dialysis method it is necessary to process 48 L of the solution in 8 hr, resulting in a requirement of 106 gm of resin. The amount of zirconium oxide resin required to remove all of the phosphate in the solution was found to be in the range of 60-80 gm. Thus the 106 gm of zirconium oxide required to adjust the pH will also meet the requirement for the removal of phosphate.









TABLE 3







Amount of Resin for 5, 10, 20 gm Urea Removed












ZP
Ammonia to
ZP
Sodium to
ZP layer size at
ZO


Layer 3
be removed
Layer 3
be removed
various pHs (gm)
Layer 4














PH
mmol
size (gm)
(mmol)
2.5
4.0
5.0
size(gm)















7.2
171
285
171
53.4114190
60-80 














6.2
171
285




80-100


7.2
342
380
342
107
228
380
60-80


6.2
342
380
127
40
85
141
106


7.2
684
456
684
213
456
760
80-100












6.2
684
456
396.7
124264 441
130









Referring now to FIG. 6 another embodiment of the resin bed of the present invention is illustrated. The resin bed 70 includes a five layer structure. The layers are similar to the resin bed 34 of FIG. 4. In this regard, the first layer 72 is zirconium phosphate, the second layer 74 is urease, the third layer 76 is zirconium phosphate, the fourth layer 78 is zirconium oxide, and the fifth layer 80 is carbon.


However, the first 72, third 76, and fourth 78 layers are slightly different than their counterparts in FIG. 4. In this regard, the first layer 72 of zirconium phosphate preferably comprises 65 grams having a pH of approximately 2.5 to about 5. The third layer of zirconium phosphate has a pH of greater than 5 and in a preferred embodiment 6.2. This layer also comprises, as in the embodiment of FIG. 4, 380 grams. The fourth layer of zirconium oxide comprises approximately 130 grams and has a pH of approximately 6.8 to about 7.5.


In the resin bed 70, once again, the first layer 72 removes the sodium but does not remove the ammonium. The first layer 72 will also adjust the pH of the solution for converting urea to ammonium by the urease layer. The pH of the solution coming out of the first layer 72 will be approximately the pH of the resin. The lower the pH of the resin, the more sodium is removed. As the solution exits the urease layer 74 and enters the third layer 76 of zirconium phosphate, the ammonium is removed. As the pH of the zirconium phosphate is increased, more ammonium is removed. A pH of at least 5 is required in order to remove the ammonium. Once again, the fourth layer 74 of zirconium oxide removes the phosphate and adjusts the pH to 7.4. The last layer 80, the carbon layer, once again removes any remaining impurities.


Referring now to FIG. 7, a further embodiment of a resin bed 82 is illustrated. In this embodiment, the first layer 84 comprises urease. The second layer 86, in an embodiment, comprises zirconium oxide at a pH of approximately 9.5 to about 12.5. Preferably 100 to 150 grams of zirconium oxide are present. The third layer 88 comprises zirconium phosphate at a pH of approximately 6.2 to about 6.5. Approximately 680 grams are present. The fourth layer 90 comprises zirconium oxide at a pH of approximately 6.8 to about 7.5 with preferably approximately 30 grams being present. The last layer 92 comprises carbon.


In the resin bed 82 the zirconium oxide layer 86 functions in the role of zirconium phosphate in the other resin beds (34 and 70). To this end, it removes the sodium. The amount of sodium removed is based on the capacity of the zirconium oxide to remove sodium. The zirconium oxide functions to remove sodium due to its high pH. On the other hand, one of the disadvantages of this structure as compared to the other resin beds (30 and 70) is that a high pH is required so that as the solution exits the second layer 86 it is at a higher pH.


Generally, it should be noted that preferably the resin beds of the present invention are structured so that urea is removed in either the first or second layers. Then preferably sodium is removed. After the sodium is removed, ammonium and then phosphate is removed. Additionally, the zirconium oxide layer functions to control the pH of the solution exiting the resin bed.


As previously noted, the resin bed of the cartridge can comprise any number of layers greater than four. It should also be noted that the layers may not have discrete boundaries, but, may be blended together. For example, it is possible to have a gradient of two materials between the zirconium oxide and the zirconium phosphate layers.


By way of example, and not limitation, real-time values for solute concentration at the inlet and outlet of cartridge 32 of the present invention will now be set forth. Due to mixing and mass transfer effects, these concentrations will be different at other locations of the system.














Parameter
Input value
Output value







Urea Concentration [mg/L]
 5-20
<10% of input value


Creatinine concentration [ ]
2  
<20% of input value


Phosphate concentration [ ]

<20% of input value


Sodium concentration [mEq/L]
122-142
122-142


Calcium concentration [mEq/L]
2.5
<0.2


Magnesium concentration [mEq/L]
0.5
<0.05


Ammonium concentration [ppm]
n.a.
<20


Aluminum concentration [ppb]
n.a.
<10









Average Values


Preferably, the time-averaged concentration of the following parameters will be maintained within the given boundaries as measured in the cartridge effluent:

















PH
7.0-7.4



Sodium [mEq/L]
127-137



Chloride [mEq/L]
85-98



Bicarbonate [mEq/L]
25-35









The pH of the effluent from the cartridge will be maintained between 6.5 and 8.0 at all times


Net Solute Removal/Addition















Parameter
Amount Removed








Urea-nitrogen
9.8 at an input concentration of 20 mg/dL











Creatinine
1.44
g



Phosphate
1.44
g



Sodium
20-60
mEq



Bicarbonate
20-60
mEq









Note: The capacity to process urea, creatinine, or phosphate depends upon the input concentration of that component. The capacity for a given component is defined by the component breakthrough, which is the amount absorbed by the cartridge when the effluent concentration exceeds a prescribed level (i.e., 10% of the input value). For safety reasons, Ammonium breakthrough levels are defined in absolute terms at 20 ppm.


As noted above, a variety of different layer structures for the resin bed are possible within the cartridge 32. In constructing the cartridge 32, the processes occurring in the cartridge must be considered. While the cartridge performs its primary task of removing urea, creatinine, phosphate, and other toxins, the by-products of this process result in changes in dialysate composition in three important respects: 1) sodium; 2) pH; and 3) bicarbonate. These three parameters are intimately related.


Sodium can be affected by three distinct processes within the cartridge:


1) Release of sodium in exchange for ammonium and other cations (calcium, magnesium, potassium). The maximum quantity of these cations to be absorbed will be about 650 mmol, consisting of about 430 mmol of ammonium and about 200 mmol of the other cations. The amount of sodium released during this exchange process is dependent on the equilibrated pH of the zirconium phosphate, the solution pH, and the concentration of cations in the dialysate.


2) pH equilibration of zirconium phosphate. In this process, sodium is exchanged for hydrogen ion in response to a solution pH which is different from the equilibrated pH of the resin. This exchange can occur in either direction, depending on whether the solution pH is above or below the equilibrated pH. It is expected that the solution pH will be greater than the equilibrated pH of the resin for much of the therapy, resulting in a net adsorption of Na+ from solution.


3) Ion exchange of zirconium oxide. As an amphoteric resin, zirconium oxide is capable of removing sodium from solution if the equilibrium pH of the zirconium oxide is sufficiently basic.


4) Adsorption of sodium by the mixed bed (demineralization) resin, if present. The amount of sodium absorbed is entirely dependent on the quantity of mixed bed resin present.


5) Liberation of alkali upon conversion of urea. Conversion of urea is a continuous process throughout the therapy. Conversion of urea may contribute up to 430 mmol alkali, and is directly related to a patient's urea load.


6) Formation of bicarbonate during the conversion of urea. Formation of bicarbonate acidifies the solution, but this effect is partially offset by venting of carbon dioxide from solutions.


7) Venting of carbon dioxide from the cartridge loop. In solution, carbon dioxide acts as an acid. Thus, removal of carbon dioxide by its movement to the gas phase and subsequent venting out of the system results in a net loss of acid from solution.


8) Buffering of the solution by zirconium phosphate. It is expected that the solution pH will be greater than the equilibrated pH of the resin resulting in a net release of acid (H+) to the solution.


9) Buffering of the solution by zirconium oxide. The zirconium oxide resin exchanges H+/OH if it is in contact with a solution having a pH different from its equilibrated pH.


Bicarbonate levels can be affected by three distinct processes within the cartridge:


1) Formation of bicarbonate during the conversion of urea. One mole of carbon dioxide/bicarbonate is formed from each mole of urea. Dissolved carbon dioxide is in equilibrium with bicarbonate according to the following relation:






pH
=

6.2
+

log







HCO

3
-




CO
2



(
aq
)









Consequently, the ratio of carbon dioxide/bicarbonate formed as a result of the urease reaction is dependent on the solution pH, with more acidic conditions favoring carbon dioxide. The overall quantity of (carbon dioxide+ bicarbonate) formed is dependent on the patient's urea load.


2) Venting of CO2 from the cartridge loop. Dissolved carbon dioxide is in equilibrium with the partial pressure of carbon dioxide in the gas phase. Thus, carbon dioxide will bubble out of solution if the solution partial pressure exceeds the partial pressure of the gas phase.


3) Adsorption of bicarbonate by zirconium oxide. zirconium oxide resin in the hydroxyl form is capable of adsorbing bicarbonate. Conversely, zirconium oxide resin in the bicarbonate form is capable of releasing bicarbonate into the solution.


The possible manipulations within the cartridge that can be made are as follows:


1) Altering the equilibrated pH of the zirconium phosphate resin. By lowering the equilibrated pH of the resin, the amount of sodium released is reduced, the average dialysate pH is lower, and the amount of carbon dioxide formed is greater. By raising the equilibrated pH of the resin, the solution pH becomes more physiologic, but the amount of sodium and bicarbonate released is increased.


2) Altering the equilibrated pH of the zirconium oxide resin or loading the resin with various counter-ions. Hydroxyl-loaded zirconium oxide results in a more physiologic solution pH, adsorption of bicarbonate from solution and increased adsorption of cations.


By way of example and not limitation, the experiments below set forth further embodiments and analysis of the invention.


Experiment No. 1

Set forth below are tests that examined the effect of modifying the equilibrium pH of zirconium phosphate on the composition of the dialysate effluent. The primary endpoints observed were pH, sodium concentration, and bicarbonate concentration. The ideal result is an effluent pH at or near the physiologic pH of 7.4, a net sodium removal of ˜50 mEq for a full-sized cartridge, and a net bicarbonate addition of ˜50 mEq for a full-size cartridge. These experiments were typically conducted at a g scale of zirconium phosphate, in a manner such that the urea concentration at ammonium breakthrough is in the expected column input range during patient therapy. At this scale, appropriate performance targets are a net sodium removal of ˜1 mEq and a net bicarbonate addition of ˜1 mEq (or 0.5 mEq/L for a 2 liter reservoir).


The resin was modified with phosphate buffer to increase the effluent pH by the following procedure. A large reservoir of 15 mM phosphate buffer was prepared using 10.8 mM dibasic sodium phosphate, 4.2 mM of monobasic sodium phosphate and 117 mM sodium chloride. The buffer was pumped through a column of resin in single pass mode. The flow rate was scaled to achieve a residence time of ˜5 minutes. The effluent pH was monitored closely, and the experiment was stopped when the effluent pH reached the desired value.


With this technique the action can be modified up to a pH of 7.2. For higher pH the same phosphate buffer is prepared and 0.1 M NaOH is added to raise the pH to the desired value.


For the modified zirconium phosphate materials, static tests were performed to determine the equilibrium capacity for ammonium. The equilibrium isotherms for the different materials are not significantly different from one another over the working concentration range [3-15 mM].


Tests were performed using a 2-liter bag as a reservoir with recirculation through columns containing the material. The bag was maintained at a uniform concentration with the aid of a shaker. The solution was pumped through the column(s) and returned to the solution bag. The bag has an outlet port with an injection site, and an inlet port that is extended 9.5 inches into the bag. The extension of the inlet port into the bag minimizes channeling between the two ports and ensures proper mixing. The solution used in these tests was Dianeal PD4 (1.5% glucose) spiked with urea and bicarbonate. precautions were taken during the filling and sampling procedures to ensure that the integrity of the system was maintained.


All the tests were performed using a urea concentration of 10 mg/dL and a sodium bicarbonate concentration of 25 mM. The initial pH for this solution was 7.4.+−0.0.2. For all the tests, 10 grams of cation material were used. Two types of urease were employed in these tests, CLEC-urease from Altus Biologics (5-20 mg) and urease from Sorb Technologies (5 g mixed with 10 g alumina). For the Sorb urease a 25 mL column was used with 8 μm filters on both ends. The urease alumina mixture was sandwiched between two lays of alumina (˜5 g each). The Sorbtech urease was packed dry. The CLEC-urease was packed wet, sandwiched between layers of Sephacryl (inert chromatography media from Sigma Chemicals) in a 10 ml column. No difference in performance was observed between the two forms of urease.


Prior to the experiment the urease was flushed with Dianeal to remove any labile or very small particle size enzyme. After the pump was started, time zero was defined by the appearance of fluid exiting the column outlet port. Samples were collected over time from both the inlet and outlet to the two-liter bag, and analyzed immediately for sodium, pH and bicarbonate using a blood gas analyzer (Chiron model 860, Chiba Corning).


Table 4 shows a summary of the relevant tests performed. Additional experiments were performed using a phosphate buffer.


From these tests it is apparent that the change in pH during the test is reduced when the pH of the resin is modified to a higher (than 6.2) pH. With an increase in resin pH the performance of the resin in terms of ammonia adsorption maintains the same, but more sodium is released into the system. The presence of the urease works in reducing the changes in pH.









TABLE 4







Results of small-scale test using urease and zirconium phosphate
















Solution
Solution


NH4+



Resin

pH,
pH,

ΔNa+
bound
ΔHCO3


pH
Date
initial
final
ΔpH
(mEq)
(mEq)
(mmol/L)





6.2
Apr. 21,
7.80
7.13
−0.67
0.5
7.3
0.5



2000


6.8
May 4,
7.41
7.21
−0.20
3.8
8.6
2.5



2000


7.1
Apr. 21,
7.25
7.47
+0.22
5.5
5.9
4.4



2000


7.4
May 4,
7.45
7.59
+0.14
5.1
6.5
2.9



2000


7.4
May 15,
7.38
7.46
+0.08
4.9
6.9
1.7



2000


7.6
May 6,
7.44
7.47
+0.03
5.5
8.8
5.3



2000


7.6
May 15,
7.36
7.56
+0.20
4.1
7.3
3.2



2000









Experiment No. 2

Experiments were conducted using urease, zirconium phosphate, and zirconium oxide in the same experimental set-up as above. Multiple columns were connected in series, with the zirconium oxide column added to the system after the cation column. The results for a test using Altus 271-6 urease, zirconium phosphate modified to a pH of 7.2 and zirconium oxide are set forth below in FIGS. 8-10. Note that the sodium balance is well maintained over the course of the test, which is a result of zirconium oxide removing sodium from the solution to counterbalance sodium released by the zirconium phosphate layer. Effluent pCO2 levels are also significantly lower in the presence of zirconium oxide. Modified zirconium oxide captures sodium, and helps maintain the sodium balance over the course of the test. The test show that zirconium phosphate modified to a pH of 7.1-7.2 performs much better than those modified to a higher pH.


Experiment No. 3

Experimental Setup:



FIG. 11 illustrates a schematic of the experimental setup used in a study to evaluate the use of ion exchange resins in peritoneal dialysis setting. The set up included two loops 100 and 102. A 15-liter bag 104 representing the total fluid body of a patient was used in the second loop 102 of the setup. Although utilizing a 40-liter bag may make a more accurate estimation of the patient body, a 15-liter bag was used due to ease of analysis. The fluid from the 15-liter bag was pumped into the lumen side 106 of the dialyzer 108 at a flow rate of 100 mL/min using a pump 110. From the outlet 112 of the lumen side 106 of the dialyzer 108, the fluid returned to the 15-liter bag 104. Concurrently, as this fluid was returning into the 15-liter bag 104, it was infused with urea, creatinine, and phosphate, at 1 mL/min, to represent the total amount of wastes being generated continuously by the patient. The 15-liter bag 102 was maintained at a constant concentration of urea-nitrogen (20 mg/dL), creatinine (6 mg/dL), and phosphate (3.1 mg/dL). The initial feed solution contains 25 mmol/L of bicarbonate, 138 mEq/L of sodium, 2.5 mEq/L of calcium and 1.0 mEq/L of magnesium.


A 4-liter bag 114 containing sodium at 132 mEq/L, calcium at 2.5 mEq/L, magnesium at 1.0 mEq/L and bicarbonate at 25 mmol/L in DI water is provided. Initially the 4-liter solution is used to prime the dialyzer 108 and a cartridge 116. As the solution exits the cartridge 116, all the toxins and also calcium and magnesium, are completely removed. Accordingly, fluid returning to the 4-liter bag 114, is infused with calcium and magnesium so as to maintain the calcium and magnesium balance in the 15-liter bag 114. Both the 4-liter 124 and the 15-liter 114 bag were well mixed and the dialyzer 118 was operated at close to zero ultra filtration.


From the 4 L bag 114, the solution flows into the shell side 128 of the dialyzer 108. The urea creatinine and phosphate diffuses from the lumen side 116 of the dialyzer 108 to the shell side 128. The solution that exits the dialyzer 108 and enters the cartridge 116 has a urea nitrogen concentration of 10 mg/dL, Creatinine concentration of 3 mg/dL and phosphate 1 mg/dL. The flowrate on either side of the dialyzer 38 is maintained at 100 ml/mm.


The cartridge 116 was constructed as set forth above. Urea creatinine and phosphate flows to the bottom 130 of the cartridge 116, which contains urease, various ion exchange resins, and carbon. As noted above, urease is an enzyme whose function is to convert toxic urea into ammonium and carbon dioxide, is the first layer in the cartridge. The middle layer comprises of two different types of ion exchange resins, zirconium phosphate (zirconium phosphate) and zirconium oxide (zirconium oxide). Zirconium phosphate, as noted above, mainly removes ammonium ions, calcium, and magnesium from the solution, while releasing hydrogen and sodium. The zirconium oxide resin removes the phosphate. Finally, a carbon layer is used to remove creatinine, uric acid, and other organics from the solution. From the top of the cartridge, fluid is then directed back into the original 4-liter bag 114.


Pursuant to this study, samples were taken at 5 different points in the above setup. Sample “1” (CIN) was taken before the fluid enters the cartridge inlet; Sample “2” (COUT) was taken as the sample exits after the cartridge; Sample “3” (4 L) was taken directly from the outflow of the 4-liter bag; Sample “4” (DOUT) was taken as the fluid comes out of the lumen of the dialyzer; Sample “5” (DIN) represents the fluid before entering the lumen inlet of the dialyzer. The sample DIN was taken from the 15 L bag 34, which is essentially well mixed and represents 15 L patient.


The above experimental setup was used to evaluate an embodiment of the cartridge of the present invention. A Redy Cartridge was obtained from Sorb Technology and used in the above experimental setup. FIG. 12 shows the various layers in the cartridge. FIG. 12a represents the Redy Cartridge, FIG. 12b represents the Redy Cartridge 1 and FIG. 12c represents the Redy Cartridge 2. The urea, creatinine and phosphate diffuse from 15 L patient bag across the dialyzer to the bottom of the cartridge. Five samples were taken from various locations as shown in FIG. 11. Samples were analyzed for pH, bicarbonate and sodium onsite. Analysis for urea, creatinine, phosphate, calcium, magnesium, chloride, lactate, and glucose were also carried out. FIGS. 13a, 13b, 13c show the pH, sodium and bicarbonate profiles. The pH in the 15 L patient bath drops from 7.546 to 6.156, bicarbonate drops from 23.2 to 0.0, sodium increases from 132.4 mEq to 135.3 mEq.


Instead of providing bicarbonate to the patient, bicarbonate is removed and sodium added. Also the pH drops and PCO2 increases. Table 4 summarizes the pH, sodium, and bicarbonate profile from this study. Overall, 44 mEq of sodium was added and all of the bicarbonate was removed. This was a net gain of 125 mEq of sodium. The cartridge does remove urea, creatinine and phosphate completely, but does not satisfy the electrolyte requirement. Thus the resins or the cartridge cannot be used in peritoneal dialysis closed loop setting or in hemodialysis applications, it cannot be used unattended. Several different combinations were evaluated that could satisfy the requirement criteria for use in the cartridge for continuous recirculation of peritoneal dialysis solution. Some of the combinations were as follows:


1—Zirconium oxide in bicarbonate form at a pH of 8.85 used with zirconium phosphate (pH=6.2) in its standard form. In this setup there were only 4 layers.


2—Zirconium phosphate with a pH of 6.5 along with zirconium oxide in the bicarbonate form at two different pHs of 10.52 and 7.33. At the higher pH, bicarbonate should be in the form of carbonate.


3—Zirconium phosphate at a pH of 6.5 was used the bicarbonate form of zirconium oxide at a pH of 9.35 and 9.83 and the hydroxyl form of the zirconium oxide at a pH of 7.14 and 7.23.


4—Zirconium phosphate at a pH of 6.49 used along with zirconium oxide in the bicarbonate form at a pH of 8.80. In this case also there were 4 layers.


5—Since zirconium oxide is an amphoteric resin, this resin needs to adsorb the Ca++ and Mg++ ions, allowing the reduction of zirconium phosphate volume to 450 ml.



FIGS. 12b and 12c represents two alternatives from the various alternatives discussed.



FIG. 12b and FIG. 12c shows the modified cartridge in the study. From equilibrium adsorption isotherm studies it was shown that at a concentration of 10 mg/dl urea nitrogen in the peritoneal dialysis solution a 600 ml resin column is required. Therefore the size of the resin in Cartridge I (FIG. 6b) is 600 ml. In FIG. 12b, (cartridge I) the 1st layer is urease, 2nd layer is zirconium phosphate (pH=6.5, volume=200 mL), 3rd layer is zirconium oxide in carbonate form (pH=9.48, volume=100 mL), 4th layer is zirconium phosphate (pH=6.5, volume=400 mL) and 5th layer is Zirconium oxide in the hydroxyl form (pH=7.38, volume=30 mL) the last layer is carbon. The zirconium oxide 3rd (High pH) is used not only to adsorb the cations, but it can also raise the pH of the zirconium phosphate resin. The counter ions used in this resin could be bicarbonate, carbonate or hydroxyl. This layer adsorbs the calcium, magnesium, thus reducing the size of the zirconium phosphate layer as it is used only to adsorb ammonia. Phosphate is also adsorbed in this layer along with the other cations. The 5th layer is zirconium oxide (pH=7.38) is used to adsorb phosphate and some sodium. But if there is no leaching of phosphate from the zirconium phosphate resin, this layer will not be required. The last layer is carbon, which again, can be placed anywhere.



FIGS. 14a, 14b & 14c represent the pH, sodium bicarbonate and profile over the entire therapy time. Table 5 summarizes the pH, bicarbonate and sodium profile. The pH in the 15-liter patient bag goes from 7.49 to 6.9. Sodium is removed from the patient (15-liter bag) approximately 57 mEq is removed. The resins are designed such that it removes sodium initially for approximately 20 minutes or so, and then the cartridge slowly adds the sodium back. Similar trend is observed in the case of bicarbonate, also approximately 22.5 mEq of bicarbonate is added back to the 15-liter patient. In this experiment, as shown in FIG. 14d 4.94 gm of urea nitrogen is processed (10.6 gm of urea) which produces 353 mmol/L of ammonia and 176 mmol of bicarbonate. In the Redy cartridge run 124 mEq of sodium was added, but in our cartridge of the present invention only 5 mEq of sodium is added back into the circulation. In the cartridge of the present invention, the net bicarbonate gain was approximately 59 mEq. But in the cartridge run bicarbonate was completely removed. The pH in the 15-liter patient loop went down to 6.15 and all the bicarbonate was removed.



FIG. 12c shows the cartridge II used in the experimental setup described in FIG. 10. The amount of zirconium phosphate was reduced to 450 ml. Layers 2 and 4 were zirconium oxide in carbonate and bicarbonate form at pH of 10.52 and 7.33. Table 6 summarizes the results from this run. In this run, the pH of the zirconium oxide in layer 2 was higher so that it has better capacity for cations. Around 97.5 mEq of sodium was removed from the 15-liter patient bag and 15 mEq of bicarbonate was removed. There was net removal of 62 mEq of sodium. An addition of 5 mEq of bicarbonate in the stream. The bicarbonate profile can be improved in this run. Here we have also reduced the amount of zirconium phosphate to remove the same amount of urea.



FIGS. 15a, 15b and 15c shows the pH bicarbonate and sodium profile over the entire therapy time. FIG. 15d shows the urea conversion. In this experiment a higher pH of the bicarbonate resin was utilized and also the zirconium phosphate resin was only 450 ml.









TABLE 5







Summary of Cartridge Test











Gain/Loss

Gain/Loss













Cartridge

4-liter Bag
15-Liter
15-Liter Bag















Time (Min.)

In
Out
4-Liter Bag
(mEq)
In
Out
(mEq)


















0
pH


7.147

7.546




480
pH
  6.153
 6.3
6.17

6.14

6.156


0
Sodium




132.4





(mEq/L)


480
Sodium
137.3
166.3
141.7
81.2
135.3
139.3
43.5  



(mEq/L)


0
Bicarbonate


23.2

23.1





(mEq/L)


480
Bicarbonate




10





(mEq/L)
















TABLE 6







Summary Cartridge 1











Gain/Loss

Gain/Loss













Cartridge

4-liter Bag
15-Liter
15-LiterBag















Time (Min.)

In
Out
4-Liter Bag
(mEq)
In
Out
(mEq)


















0
pH


6.99

7.49




480
pH
 6.9
  7.09
7.06

6.9
  6.997



0
Sodium


124.4

137





(mEq/L)


480
Sodium
135.4
142.6
139.9
62
133.2
137.2
57



(mEq/L)


0
Bicarbonate


22

23.4





(mEq/L)


480
Bicarbonate
 28.4
 31.8
31.1
  36.4
24.9
 26.4
  22.5



(mEq/L)
















TABLE 7







Summary Cartridge II















Gain/Loss

Gain/Loss



Cartridge

4-liter Bag
15-Liter
15-Liter Bag















Time (Min.)

In
Out
4-Liter Bag
(mEq)
In
Out
(mEq)


















0
pH


7.08

7.42




480
pH
  7.106
  7.235
7.2

7.036
  7.122



0
Sodium


126

136.60





(mEq/L)


480
Sodium
132.6
139.9
135.3
37.2
130.1
133.7
99



(mEq/L)


0
Bicarbonate


22

23.5





(mEq/L)


480
Bicarbonate
 26.2
28 
26.9
19.6
22.5
24 
−15 



(mEq/L)









It should be understood that various changes and modifications to the presently preferred embodiments described herein will be apparent to those skilled in the art. Such changes and modifications can be made without departing from the spirit and scope of the present subject matter and without diminishing its intended advantages. It is therefore intended that such changes and modifications be covered by the appended claims.

Claims
  • 1. A dialysis system comprising: a dialysate supply container;a dialysate loop;a dialysate pump positioned and arranged to fluidly communicate dialysate from the dialysate supply container along the dialysate loop;a supply of concentrate;a concentrate pump for pumping concentrate from the supply of concentrate; anda sorbent cartridge for cleaning used dialysate flowing in the dialysate loop, wherein the sorbent cartridge includes (i) a layer comprising urease, a layer comprising zirconium oxide, a layer comprising zirconium phosphate, and a layer comprising carbon, and (ii) a concentrate port for receiving concentrate from the supply of concentrate.
  • 2. The dialysis system of claim 1, wherein the sorbent cartridge includes an inlet cap, an outlet cap, and a resin bed located between the inlet cap and the outlet cap, the resin bed structured and arranged to remove waste from dialysate flowing in the dialysate loop.
  • 3. The dialysis system of claim 2, wherein the inlet cap is located at a bottom of the sorbent cartridge.
  • 4. The dialysis system of claim 2, wherein the sorbent cartridge includes an open-headed chamber located upstream of the resin bed, the open-headed chamber structured and arranged to distribute flow evenly across a cross-section of the sorbent cartridge.
  • 5. The dialysis system of claim 2, wherein the sorbent cartridge includes an open-headed chamber located downstream from the resin bed, the open-headed chamber structured and arranged to maintain an even fluid velocity throughout the resin bed.
  • 6. The dialysis system of claim 2, wherein the sorbent cartridge includes (i) a first open-headed chamber located upstream of the resin bed, the first open-headed chamber structured and arranged to distribute flow evenly across a cross-section of the sorbent cartridge, and (ii) a second-open headed chamber located downstream from the resin bed, the second open-headed chamber structured and arranged to maintain an even fluid velocity throughout the resin bed.
  • 7. The dialysis system of claim 6, which includes a gas separation chamber located downstream from the second open-headed chamber.
  • 8. The dialysis system of claim 1, wherein the sorbent cartridge includes a gas separation chamber.
  • 9. The dialysis system of claim 8, wherein the sorbent cartridge includes a gas vent for venting gas from the gas separation chamber.
  • 10. The dialysis system of claim 9, wherein the gas vent includes a filter.
  • 11. The dialysis system of claim 8, wherein the sorbent cartridge includes a dialysate fluid outlet and the gas separation chamber includes a barrier structured and arranged to produce a flow pattern that restricts gas from being drawn into the dialysate fluid outlet.
  • 12. The dialysis system of claim 1, wherein the sorbent cartridge includes an outlet cap, the outlet cap including (i) a dialysate fluid outlet, and (ii) a gas vent for venting gas from the gas separation chamber.
  • 13. The dialysis system of claim 1, which includes an ultrafiltration collection container fluidly communicating with the dialysate loop.
  • 14. A dialysis system comprising: a dialysate supply container;a dialysate loop;a dialysate pump positioned and arranged to fluidly communicate dialysate from the dialysate supply container along the dialysate loop;a supply of concentrate;a concentrate pump in fluid communication with the supply of concentrate for supplying concentrate to the dialysate loop;a sorbent cartridge for cleaning used dialysate flowing in the dialysate loop, wherein the sorbent cartridge includes a layer comprising urease, a layer comprising zirconium oxide, a layer comprising zirconium phosphate, and a layer comprising carbon; anda gas vent located downstream from the sorbent cartridge for venting gas from the dialysate loop.
  • 15. The dialysis system of claim 14, which includes an air sensor in operable communication with the dialysate loop for detecting air in the dialysate loop.
  • 16. The dialysis system of claim 14, wherein the sorbent cartridge includes (i) a dialysate fluid inlet, (ii) an outlet cap and (iii) a resin bed located between the dialysate fluid inlet and the outlet cap.
  • 17. The dialysis system of claim 14, which includes an ultrafiltration collection container fluidly communicating with the dialysate loop.
  • 18. The dialysis system of claim 14, wherein the concentrate is pumped into the dialysate loop at a location downstream from the sorbent cartridge.
  • 19. The dialysis system of claim 1, wherein the concentrate is pumped into the dialysate loop at a location downstream from the sorbent cartridge.
  • 20. The dialysis system of claim 1, which is configured to perform peritoneal dialysis or hemodialysis.
  • 21. The dialysis system of claim 14, which is configured to perform peritoneal dialysis or hemodialysis.
  • 22. A dialysis system comprising: a dialysate supply container;a dialysate loop;a dialysate pump positioned and arranged to fluidly communicate dialysate from the dialysate supply container along the dialysate loop;a supply of concentrate;a concentrate pump in fluid communication with the supply of concentrate for supplying concentrate to the dialysate loop; anda sorbent cartridge for cleaning used dialysate flowing in the dialysate loop, wherein the sorbent cartridge includes a layer comprising urease, a layer comprising zirconium oxide, a layer comprising zirconium phosphate, and a layer comprising carbon, the sorbent cartridge further including a gas separation chamber having a gas vent for venting gas from the gas separation chamber.
  • 23. A dialysis system comprising: a dialysate supply container;a dialysate loop;a dialysate pump positioned and arranged to fluidly communicate dialysate from the dialysate supply container along the dialysate loop;a supply of concentrate;a concentrate pump in fluid communication with the supply of concentrate for supplying concentrate to the dialysate loop; anda sorbent cartridge for cleaning used dialysate flowing in the dialysate loop, wherein the sorbent cartridge includes a layer comprising urease, a layer comprising zirconium oxide, a layer comprising zirconium phosphate, and a layer comprising carbon, the sorbent cartridge further including an outlet cap, the outlet cap including (i) a dialysate fluid outlet, (ii) a gas vent for venting gas from the gas separation chamber, and (iii) a concentrate port for receiving concentrate from the supply of concentrate.
CROSS-REFERENCE TO RELATED APPLICATIONS

This application is a continuation of U.S. patent application Ser. No. 14/666,659, filed Mar. 24, 2015, which is a continuation of U.S. patent application Ser. No. 13/920,843, filed Jun. 18, 2013, now U.S. Pat. No. 9,393,356, issued Jul. 19, 2016, which is a divisional application of U.S. patent application Ser. No. 13/281,675, filed on Oct. 26, 2011, now U.S. Pat. No. 8,491,517, issued Jul. 23, 2013, which is a divisional application of U.S. patent application Ser. No. 12/465,214, filed on May 13, 2009, now U.S. Pat. No. 8,066,658, issued Nov. 29, 2011, which is a continuation of U.S. patent application Ser. No. 11/774,359, filed on Jul. 6, 2007, now U.S. Pat. No. 7,955,290, which is a divisional application of U.S. patent application Ser. No. 09/990,673, filed Nov. 13, 2001, now U.S. Pat. No. 7,241,272, issued Jul. 10, 2007, the entire contents of each of which are expressly incorporated herein by reference.

US Referenced Citations (350)
Number Name Date Kind
2529028 Landon Jul 1947 A
2122509 Beliaeff Jul 1948 A
3332737 Krause Jul 1967 A
3388803 Scott Jun 1968 A
3463728 Kolobow et al. Aug 1969 A
3485245 Lahr et al. Dec 1969 A
3490479 Mott et al. Jan 1970 A
3528550 Cappelen, Jr. Sep 1970 A
3545438 De Vries Dec 1970 A
3580712 Mumford May 1971 A
3608729 Haselden Sep 1971 A
3617545 Dabois et al. Nov 1971 A
3619423 Galletti et al. Nov 1971 A
3667612 Leonard Jun 1972 A
3669878 Marantz et al. Jun 1972 A
3669880 Marantz et al. Jun 1972 A
3682817 Marx Aug 1972 A
3697418 Johnson Oct 1972 A
3703959 Raymond Nov 1972 A
3707967 Kitrilakis et al. Jan 1973 A
3727612 Sayers et al. Apr 1973 A
3730183 Goldsmith et al. May 1973 A
3774672 Lichtenstein Nov 1973 A
3774762 Lichtenstein Nov 1973 A
3799873 Brown Mar 1974 A
3809241 Alvine May 1974 A
3825493 Brown et al. Jul 1974 A
3827975 Bizot et al. Aug 1974 A
3850835 Marantz et al. Nov 1974 A
3865726 Chibata et al. Feb 1975 A
3878564 Yao et al. Apr 1975 A
3884808 Scott May 1975 A
3911915 Seifter et al. Oct 1975 A
3926797 Gigou et al. Dec 1975 A
3939069 Granger et al. Feb 1976 A
3979284 Granger et al. Sep 1976 A
3989622 Marantz et al. Nov 1976 A
4000072 Sato et al. Dec 1976 A
4031010 Nose Jun 1977 A
4036747 Hori et al. Jul 1977 A
4081372 Atkin et al. Mar 1978 A
4096059 Pinkerton Jun 1978 A
4115259 Bigi Sep 1978 A
4118314 Yoshida Oct 1978 A
4161264 Malmgren et al. Jul 1979 A
4173537 Newhart et al. Nov 1979 A
4180460 Calari Dec 1979 A
4190047 Jacobsen et al. Feb 1980 A
4190536 Grimsrud Feb 1980 A
4191646 Larsson et al. Mar 1980 A
4192748 Hyden Mar 1980 A
4194536 Stine et al. Mar 1980 A
4209391 Lipps et al. Jun 1980 A
4209392 Wallace Jun 1980 A
4212738 Henne Jul 1980 A
4213859 Smakman et al. Jul 1980 A
4229299 Savitz et al. Oct 1980 A
4240408 Schael Dec 1980 A
4244816 Vogler et al. Jan 1981 A
4247393 Wallace Jan 1981 A
4256718 McArthur et al. Mar 1981 A
4267040 Schal May 1981 A
4267047 Henne et al. May 1981 A
4269708 Bounomini et al. May 1981 A
4276175 Bower Jun 1981 A
4293762 Ogawa Oct 1981 A
4303521 Lehmann Dec 1981 A
4313831 Lehmann Feb 1982 A
4338190 Kraus et al. Jul 1982 A
4360507 McArthur et al. Nov 1982 A
4364747 Blackshear et al. Dec 1982 A
4366061 Papanek et al. Dec 1982 A
4381003 Buoncristiani Apr 1983 A
4386634 Stasz et al. Jun 1983 A
4460555 Thompson Jul 1984 A
4464172 Lichtenstein Aug 1984 A
4464563 Jewett Aug 1984 A
4468329 Shaldon et al. Aug 1984 A
4473449 Michaels et al. Sep 1984 A
4477342 Allan et al. Oct 1984 A
4498900 Bouncristiani Feb 1985 A
4530759 Schal Jul 1985 A
4532414 Shah et al. Jul 1985 A
4542015 Smakman et al. Sep 1985 A
4581141 Ash Apr 1986 A
4586920 Peabody May 1986 A
4614590 Rath et al. Sep 1986 A
4618343 Polashegg Oct 1986 A
RE32303 Lasker et al. Dec 1986 E
4650458 Dehlberg et al. Mar 1987 A
4650857 May Mar 1987 A
4661246 Ash Apr 1987 A
4678460 Rosner Jul 1987 A
4680445 Ogawa Jul 1987 A
4684460 Issautier Aug 1987 A
4702829 Polaschegg et al. Oct 1987 A
4703913 Hunkapiller Nov 1987 A
4708802 Rath et al. Nov 1987 A
4711715 Polaschegg Dec 1987 A
4715959 Allan et al. Dec 1987 A
4718890 Peabody Jan 1988 A
4735609 Comeau et al. Apr 1988 A
4747822 Peabody May 1988 A
4747950 Guinn May 1988 A
4756706 Kerns et al. Jul 1988 A
4765907 Scott Aug 1988 A
4767399 Bollish Aug 1988 A
4769134 Allan et al. Sep 1988 A
4769151 Shouldice Sep 1988 A
4770769 Schael Sep 1988 A
4804474 Blum Feb 1989 A
4804950 Moon et al. Feb 1989 A
4828543 Weiss et al. May 1989 A
4834888 Polaschegg May 1989 A
4838865 Flank et al. Jun 1989 A
4844074 Kurucz Jul 1989 A
4847470 Bakke Jul 1989 A
4857199 Cortial Aug 1989 A
4873623 Lane et al. Oct 1989 A
4898578 Rubalcaba et al. Feb 1990 A
4906816 van Leerdam Mar 1990 A
4914624 Dunthorn Apr 1990 A
4916441 Gombrich Apr 1990 A
4935125 Era et al. Jun 1990 A
4950259 Geary et al. Aug 1990 A
4971700 Tsuii et al. Nov 1990 A
4976683 Gauthier et al. Dec 1990 A
4997570 Polaschegg Mar 1991 A
5004459 Peabody et al. Apr 1991 A
5056059 Tivig et al. Oct 1991 A
5073167 Carr et al. Dec 1991 A
5114580 Ahmad et al. May 1992 A
5125069 O'Boyle Jun 1992 A
5141492 Dadson et al. Aug 1992 A
5141493 Jacobson et al. Aug 1992 A
5152671 Harant Oct 1992 A
5173125 Felding Dec 1992 A
5180896 Gibby et al. Jan 1993 A
5211849 Kitaevich et al. May 1993 A
5227820 Miyashita et al. Jul 1993 A
5245693 Ford et al. Sep 1993 A
5282783 Lindsay Feb 1994 A
5284470 Beltz Feb 1994 A
5336173 Folden Aug 1994 A
5338293 Jeppsson et al. Aug 1994 A
5350357 Kamen et al. Sep 1994 A
5366630 Chevallet Nov 1994 A
5370674 Farrell Dec 1994 A
5376263 Fischel Dec 1994 A
5381510 Ford et al. Jan 1995 A
5408576 Bishop Apr 1995 A
5420962 Bakke May 1995 A
5421823 Kamen et al. Jun 1995 A
5438510 Bryant et al. Aug 1995 A
5470483 Bene et al. Nov 1995 A
5474683 Bryant et al. Dec 1995 A
5498338 Kruger et al. Mar 1996 A
5522998 Polaschegg Jun 1996 A
5536412 Ash Jul 1996 A
5542919 Simon et al. Aug 1996 A
5578223 Bene et al. Nov 1996 A
5614677 Wansiedler et al. Mar 1997 A
5641405 Keshaviah et al. Jun 1997 A
5643201 Peabody et al. Jul 1997 A
5645734 Kenley et al. Jul 1997 A
5660722 Nederlof Aug 1997 A
5683381 Carr et al. Nov 1997 A
5685988 Malchesky Nov 1997 A
5685989 Krivitski et al. Nov 1997 A
5690614 Carr et al. Nov 1997 A
5698090 Bene et al. Dec 1997 A
5702597 Chevallet et al. Dec 1997 A
5722947 Jeppsson et al. Mar 1998 A
5724478 Thweatt Mar 1998 A
5725775 Bene et al. Mar 1998 A
5729653 Magliochetti et al. Mar 1998 A
5730712 Falkvall et al. Mar 1998 A
5762782 Kenley et al. Jun 1998 A
5774042 Johnston Jun 1998 A
5776345 Truitt et al. Jul 1998 A
5783085 Fischel Jul 1998 A
5788846 Sternby Aug 1998 A
5790752 Anglin et al. Aug 1998 A
5816779 Lawless et al. Oct 1998 A
5836908 Beden et al. Nov 1998 A
5846419 Nederlof Dec 1998 A
5858238 McRea et al. Jan 1999 A
5863421 Peter, Jr. et al. Jan 1999 A
5873853 Keilman Feb 1999 A
5875282 Jordan et al. Feb 1999 A
5876611 Shettigar Mar 1999 A
5902336 Mishkin May 1999 A
5910252 Truitt et al. Jun 1999 A
5919357 Wilkins et al. Jul 1999 A
5919369 Ash Jul 1999 A
5921951 Morris Jul 1999 A
5925011 Faict et al. Jul 1999 A
5938634 Packard Aug 1999 A
5944684 Roberts et al. Aug 1999 A
5960160 Clark et al. Sep 1999 A
5980481 Gorsuch Nov 1999 A
5984891 Keilman et al. Nov 1999 A
5989238 Ginsburg Nov 1999 A
5989423 Kamen et al. Nov 1999 A
6036668 Mathis Mar 2000 A
6042784 Wamsiedler et al. Mar 2000 A
6069343 Kolowich May 2000 A
6074359 Keshaviah et al. Jun 2000 A
6077443 Goldau Jun 2000 A
6110384 Goux et al. Aug 2000 A
6126831 Goldau et al. Oct 2000 A
6129699 Haight et al. Oct 2000 A
6139528 Kistner et al. Oct 2000 A
6139748 Ericson et al. Oct 2000 A
6142974 Kistner et al. Nov 2000 A
6146359 Carr et al. Nov 2000 A
6168578 Diamond Jan 2001 B1
6175688 Cassidy et al. Jan 2001 B1
6193684 Burbank et al. Feb 2001 B1
6196992 Keilman et al. Mar 2001 B1
6210361 Kamen et al. Apr 2001 B1
6220299 Arvidsson et al. Apr 2001 B1
6228047 Dadson May 2001 B1
6229957 Baker May 2001 B1
6234991 Gorsuch May 2001 B1
6236809 Cassidy et al. May 2001 B1
6245039 Brugger et al. Jun 2001 B1
6234992 Haight et al. Jul 2001 B1
6254567 Trea et al. Jul 2001 B1
6260715 Simard et al. Jul 2001 B1
6261261 Gordon Jul 2001 B1
6261809 Bertling et al. Jul 2001 B1
6280632 Polaschegg Aug 2001 B1
6287516 Matson et al. Sep 2001 B1
6290669 Zicherman Sep 2001 B1
6293921 Shinmoto et al. Sep 2001 B1
6302653 Bryant et al. Oct 2001 B1
6409699 Ash Jun 2002 B1
6447491 Lord Sep 2002 B1
6491656 Morris Dec 2002 B1
6495366 Briggs Dec 2002 B1
6561997 Weitzel et al. May 2003 B1
6572576 Brugger et al. Jun 2003 B2
6572641 Brugger et al. Jun 2003 B2
6579253 Burbank et al. Jun 2003 B1
6582385 Burbank et al. Jun 2003 B2
6509482 Burbank et al. Jul 2003 B2
6585682 Haraldsson et al. Jul 2003 B1
6602502 Strahilevitz Aug 2003 B1
6607669 Schick Aug 2003 B2
6620120 Landry et al. Sep 2003 B2
6638477 Treu et al. Oct 2003 B1
6638478 Treu et al. Oct 2003 B1
6649063 Brugger et al. Nov 2003 B2
6666842 Sakai Dec 2003 B1
6702561 Stillig et al. Mar 2004 B2
6733676 Takai May 2004 B2
6743201 Doenig et al. Jun 2004 B1
6746606 Pfeil et al. Jun 2004 B2
6746607 Vijayalakshmi et al. Jun 2004 B1
6752928 Pfeil et al. Jun 2004 B2
6758975 Peabody et al. Jul 2004 B2
6776912 Baurmeister Aug 2004 B2
6780322 Bissler et al. Aug 2004 B1
6821441 Pedrini et al. Nov 2004 B2
6830553 Burbank et al. Dec 2004 B1
6843779 Andrysiak et al. Jan 2005 B1
6852090 Burbank et al. Feb 2005 B2
6890157 Pfeil et al. May 2005 B2
6918886 Baurmeister Jul 2005 B1
6955655 Burbank et al. Oct 2005 B2
6960179 Gura Nov 2005 B2
6976973 Ruddell et al. Dec 2005 B1
6979309 Burbank et al. Dec 2005 B2
7008403 Mallett Mar 2006 B1
7074332 Summerton et al. Jul 2006 B2
7112273 Weigel et al. Sep 2006 B2
7208092 Micheli Apr 2007 B2
7238164 Childers et al. Jul 2007 B2
7241272 Karoor et al. Jul 2007 B2
7744554 Howard Jun 2010 B2
7867189 Childers et al. Jan 2011 B2
7867214 Childers et al. Jan 2011 B2
7922686 Childers et al. Apr 2011 B2
7922911 Micheli Apr 2011 B2
8034161 Gura et al. Oct 2011 B2
8137553 Fulkerson et al. Mar 2012 B2
8206338 Childers et al. Jun 2012 B2
8357113 Childers et al. Jan 2013 B2
8425780 Beiriger Apr 2013 B2
8597227 Childers et al. Dec 2013 B2
8679054 Childers et al. Mar 2014 B2
8740836 Childers et al. Jun 2014 B2
8740837 Childers et al. Jun 2014 B2
8815095 Micheli Aug 2014 B2
8992462 Childers et al. Mar 2015 B2
8998839 Childers et al. Apr 2015 B2
9283312 Childers et al. Mar 2016 B2
9764074 Childers et al. Sep 2017 B1
9795729 Childers et al. Oct 2017 B2
9814820 Childers et al. Nov 2017 B2
10232103 Karoor Mar 2019 B1
20010021817 Brugger et al. Sep 2001 A1
20010032818 Nikaido et al. Oct 2001 A1
20010037079 Burbank et al. Nov 2001 A1
20010041873 Dopper et al. Nov 2001 A1
20010041892 Burbank et al. Nov 2001 A1
20010045395 Kitaevich et al. Nov 2001 A1
20020017489 Utterberg Feb 2002 A1
20020041825 Scheunert et al. Apr 2002 A1
20020072718 Brugger et al. Jun 2002 A1
20020082728 Mueller et al. Jun 2002 A1
20020103453 Burbank et al. Aug 2002 A1
20020147423 Burbank et al. Oct 2002 A1
20020187940 Masuda et al. Dec 2002 A1
20020197250 Brady et al. Dec 2002 A1
20030000876 Kawaguchi Jan 2003 A1
20030010717 Burbank et al. Jan 2003 A1
20030010718 Burbank et al. Jan 2003 A1
20030018290 Brugger et al. Jan 2003 A1
20030036719 Giacomelli et al. Feb 2003 A1
20030105424 Karoor et al. Jun 2003 A1
20040158189 Tonelli et al. Aug 2004 A1
20040238416 Burbank et al. Dec 2004 A1
20040238418 Ikeda Dec 2004 A1
20040240349 Brugger et al. Dec 2004 A1
20040243046 Brugger et al. Dec 2004 A1
20040243047 Brugger et al. Dec 2004 A1
20040243048 Brugger et al. Dec 2004 A1
20040243050 Treu et al. Dec 2004 A1
20040245161 Treu et al. Dec 2004 A1
20040247185 Weaver et al. Dec 2004 A1
20040249331 Burbank et al. Dec 2004 A1
20040267184 Burbank et al. Dec 2004 A1
20050000868 Weigel et al. Jan 2005 A1
20050004502 O'Mahony et al. Jan 2005 A1
20050010158 Brugger et al. Jan 2005 A1
20050011823 Delnevo et al. Jan 2005 A1
20050020958 Paolini et al. Jan 2005 A1
20050020959 Brugger et al. Jan 2005 A1
20050020960 Brugger et al. Jan 2005 A1
20050101901 Gura May 2005 A1
20050102028 Arnin et al. May 2005 A1
20050230292 Beden et al. Oct 2005 A1
20060138049 Stahl Jun 2006 A1
20070038191 Burbank et al. Feb 2007 A1
20110297593 Kelly et al. Dec 2011 A1
20130256227 Kelly et al. Oct 2013 A1
20140001112 Karoor et al. Jan 2014 A1
20140190886 Pudil et al. Jul 2014 A1
Foreign Referenced Citations (116)
Number Date Country
2002 033 Aug 1970 DE
29 01 628 Jul 1980 DE
31 22 756 Jun 1982 DE
3110128 Sep 1982 DE
33 07 830 Jun 1984 DE
210 425 Jun 1984 DE
40 03 452 Aug 1991 DE
42 08 054 Oct 1992 DE
41 22 754 Jan 1993 DE
19830928 May 1999 DE
19814695 Oct 1999 DE
19828923 Jan 2000 DE
198 54 338 Jun 2000 DE
10011208 Sep 2001 DE
19814695 Sep 2001 DE
10100146 Jul 2002 DE
64393 Nov 1982 EP
0143341 Jun 1985 EP
152717 Aug 1985 EP
0165751 Dec 1985 EP
0166920 Jan 1986 EP
0233848 Aug 1987 EP
0306241 Mar 1989 EP
0373455 Jun 1990 EP
0222709 May 1991 EP
0243547 Jul 1991 EP
0451429 Oct 1991 EP
0490212 Jun 1992 EP
0402505 Dec 1993 EP
0623357 Nov 1994 EP
0722744 Jul 1996 EP
0498382 Nov 1996 EP
0778033 Nov 1996 EP
0796998 Sep 1997 EP
0575512 May 1998 EP
0928615 Jul 1999 EP
0956876 Nov 1999 EP
980685 Feb 2000 EP
0659092 Oct 2000 EP
0659091 Dec 2000 EP
1097724 May 2001 EP
0847769 Aug 2001 EP
7331918 Feb 1979 FR
2585251 Jan 1987 FR
2122509 Jan 1984 GB
2124511 Feb 1984 GB
2246718 Feb 1992 GB
51-015360 May 1976 JP
52-026076 Jul 1977 JP
55-000175 Jan 1980 JP
55-32384 Mar 1980 JP
55-122559 Sep 1980 JP
59-029264 Feb 1984 JP
61-25564 Feb 1986 JP
61-119275 Jun 1986 JP
61-143074 Jun 1986 JP
92002060 Jan 1992 JP
4348757 Mar 1992 JP
07-035413 Feb 1995 JP
07-299455 Nov 1995 JP
8029224 Feb 1996 JP
96029224 Feb 1996 JP
9327511 Dec 1997 JP
10085324 Apr 1998 JP
11137672 May 1999 JP
11226121 Aug 1999 JP
200084071 Mar 2000 JP
200120483 Dec 2000 JP
2004-205146 Jul 2004 JP
2004-209103 Jul 2004 JP
2006-500968 Jan 2006 JP
2011-172961 Aug 2011 JP
1012918 Mar 1981 SE
1344362 Jun 1984 SE
9420158 Sep 1994 WO
9502559 Jan 1995 WO
9535124 Dec 1995 WO
9747337 Jun 1997 WO
9817333 Apr 1998 WO
9822165 May 1998 WO
9832477 Jul 1998 WO
9903519 Jan 1999 WO
9906082 Feb 1999 WO
9942150 Aug 1999 WO
0009182 Feb 2000 WO
0020050 Apr 2000 WO
0020052 Apr 2000 WO
0031967 Jun 2000 WO
0050143 Aug 2000 WO
0051701 Sep 2000 WO
0057925 Oct 2000 WO
0057926 Oct 2000 WO
0057927 Oct 2000 WO
0057928 Oct 2000 WO
0064510 Nov 2000 WO
0124849 Apr 2001 WO
0137786 May 2001 WO
0137894 May 2001 WO
0137895 May 2001 WO
0137900 May 2001 WO
0141831 Jun 2001 WO
0141832 Jun 2001 WO
0142758 Jun 2001 WO
0145769 Jun 2001 WO
0141833 Jun 2001 WO
0147576 Jul 2001 WO
0147581 Jul 2001 WO
02043859 Jun 2002 WO
02070042 Sep 2002 WO
03041764 May 2003 WO
04082731 Sep 2004 WO
05042065 May 2005 WO
05044339 May 2005 WO
05044340 May 2005 WO
06105605 Oct 2006 WO
07074425 Jul 2007 WO
Non-Patent Literature Citations (41)
Entry
U.S. Appl. No. 13/213,358, filed Aug. 19, 2011, Kelly et al.
U.S. Appl. No. 13/213,676, filed Aug. 19, 2011, Lo et al.
U.S. Appl. No. 13/213,692, filed Aug. 19, 2011, Lo et al.
U.S. Appl. No. 13/213,812, filed Aug. 19, 2011, Lo et al.
U.S. Appl. No. 13/213,737, filed Aug. 19, 2011, Childers et al.
U.S. Appl. No. 13/213,727, filed Aug. 19, 2011, Childers et al.
U.S. Appl. No. 13/213,707, filed Aug. 19, 2011, Childers et al.
U.S. Appl. No. 14/666,966, filed Mar. 24, 2015, Childers et al.
“Fresnius 90/2 Peritoneal Therapy Cylcer” Article, written by Fresenius USA, dated Jul. 1993.
International Search Report and the Written Opinion for International Application No. PCT/US2008/064086 dated Jan. 27, 2009.
Japanese Office Action for Japanese Appln. No. 2009-527618.
Japanese Office Action dated Dec. 20, 2012 for Japanese Appln. No. 2010-514907.
Japanese Office Action dated Jun. 13, 2013 for Japanese Appln. No. 2011-100145.
Japanese Office Action dated Feb. 18, 2014, for Japanese Appln. No. 2013-051434.
Japanese Office Action dated Jan. 10, 2014 for Japanese Appln. No. 2013-000322.
Japanese Office Action dated Jan. 30, 2014 for Japanese Appln. No. 2011-163710.
Japanese Office Action dated Oct. 1, 2014 for Japanese Appln. No. 2013-110584.
English translation of Japanese Office Action dated Apr. 1, 2014, for Japanese Appln. No. 2013-110584.
European Search Report for European Application No. 11 07 5124 dated Mar. 16, 2012.
European Search Report for European Application No. 11 07 5125 dated Mar. 26, 2012.
European Search Report for European Application No. 11 07 5126 dated Mar. 22, 2012.
European Search Report for European Application No. 11 07 5127 dated Mar. 28, 2012.
European Search Report for European Application No. 11 07 5128 dated Apr. 3, 2012.
European Search Report for European Application No. 11 07 5129 dated Mar. 29, 2012.
European Office Action for European Appln. No. 11075126.0.
European Office Action dated Apr. 18, 2013 for European Appln. No. 11075127.8.
European Office Action dated Jun. 6, 2013 for European Appln. No. 11075125.2.
European Office Action received dated Aug. 20, 2013 for European Appln. No. 11075128.6.
European Office Action received by foreign associate dated Sep. 26, 2013 for European Appln. No. 11075129.4.
European Office Action received by foreign associate dated Sep. 30, 2013 for European Appln. No. 11075130.2.
European Office Action received by foreign associate dated Sep. 30, 2013 for European Appln. No. 11185112.7.
European Office Action received by foreign associate dated Nov. 10, 2014 for European Appln. No. 11185112.7.
European Office Action received by foreign associate dated Sep. 26, 2013 for European Appln. No. 11185090.5.
European Office Action dated Oct. 6, 2014 for European Appln. No. 11185090.5-1651.
Extended European Search Report dated Dec. 20, 2011 for European Appln. No. 11185112.7.
Extended European Search Report dated Dec. 22, 2011 for European Appln. No. 11185090.5.
Extended European Search Report dated Mar. 15, 2012 for European Appln. No. 11075130.2.
Non-Final Office Action dated Nov. 26, 2014 for U.S. Appl. No. 13/213,350.
Manns et al., “The acu-menTM: A new device for continuous renal replacement therapy in acute renal failure”, Kidney International, 1998, pp. 266-274, vol. 54.
Roberts et al., “REDY Sorbent Hemodialysis”, chapter 11, pp. 146-163.
Innovative Peritoneal Dialysis: Flow-Thru and Dialysate Regeneration; Martin Roberts, Stephen R. Ash, and David B. N. Lee; ASAIO Journal 1999, Scholarly Review, pp. 372-378.
Related Publications (1)
Number Date Country
20190167881 A1 Jun 2019 US
Divisions (3)
Number Date Country
Parent 13281675 Oct 2011 US
Child 13920843 US
Parent 12465214 May 2009 US
Child 13281675 US
Parent 09990673 Nov 2001 US
Child 11774359 US
Continuations (3)
Number Date Country
Parent 14666659 Mar 2015 US
Child 16269923 US
Parent 13920843 Jun 2013 US
Child 14666659 US
Parent 11774359 Jul 2007 US
Child 12465214 US