US20170130183A1 - Device for Cell Culturing and Processing - Google Patents
Device for Cell Culturing and Processing Download PDFInfo
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- US20170130183A1 US20170130183A1 US14/434,661 US201414434661A US2017130183A1 US 20170130183 A1 US20170130183 A1 US 20170130183A1 US 201414434661 A US201414434661 A US 201414434661A US 2017130183 A1 US2017130183 A1 US 2017130183A1
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Images
Classifications
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12M—APPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
- C12M23/00—Constructional details, e.g. recesses, hinges
- C12M23/42—Integrated assemblies, e.g. cassettes or cartridges
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12M—APPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
- C12M23/00—Constructional details, e.g. recesses, hinges
- C12M23/34—Internal compartments or partitions
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12M—APPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
- C12M23/00—Constructional details, e.g. recesses, hinges
- C12M23/40—Manifolds; Distribution pieces
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12M—APPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
- C12M29/00—Means for introduction, extraction or recirculation of materials, e.g. pumps
- C12M29/04—Filters; Permeable or porous membranes or plates, e.g. dialysis
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12M—APPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
- C12M35/00—Means for application of stress for stimulating the growth of microorganisms or the generation of fermentation or metabolic products; Means for electroporation or cell fusion
- C12M35/02—Electrical or electromagnetic means, e.g. for electroporation or for cell fusion
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12M—APPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
- C12M41/00—Means for regulation, monitoring, measurement or control, e.g. flow regulation
- C12M41/30—Means for regulation, monitoring, measurement or control, e.g. flow regulation of concentration
- C12M41/36—Means for regulation, monitoring, measurement or control, e.g. flow regulation of concentration of biomass, e.g. colony counters or by turbidity measurements
-
- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12M—APPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
- C12M41/00—Means for regulation, monitoring, measurement or control, e.g. flow regulation
- C12M41/46—Means for regulation, monitoring, measurement or control, e.g. flow regulation of cellular or enzymatic activity or functionality, e.g. cell viability
Definitions
- the present invention describes a device used in the field of biological and genetic engineering, especially a device for cell cultivation, cell transformation and biological experiments.
- the current laboratory practice accomplishes the above steps through a sequence of manual operations on small batches of cells.
- the commonly used traditional experimental instruments include: test tube, shaker flask, shaking table, Petri dish, cuvette, syringe, pipette, centrifuge, membrane filter, and so on.
- the present invention provides a compact, flexible and automated device for cell culturing and processing, which, may be used for different experimental projects, substitute repetitive manual handling, save time and labor, avoid wasting of raw materials, and minimize the risk of human exposure to potentially dangerous substances.
- the technical solution for solving the above problem by the present invention is a device for cell culturing and processing, comprising at least one central distribution compartment, at least one incubation compartment; at least one processing compartment, a number of ducts to transfer fluids between said compartments, wherein a distribution cavity and a piston capable of moving back and forth in said distribution cavity for altering the operational volume of said distribution cavity are provided within said central distribution compartment, and a distribution valve controlling the connection between said distribution cavity and said ducts is provided at one end of said distribution cavity within the distribution compartment.
- the cells grow and multiply in the incubation compartment.
- liquid can be transferred between the compartments by moving the piston within the distribution cavity.
- the distribution cavity can be connected to any of the processing compartments, which offer the possibility to accomplish tasks including removing cells from the nutrition medium and re-suspending them in another liquid, cooling, heating, optical density measurement, conductivity measurement, electro-transformation, and exposure to electro-magnetic radiation.
- said central distribution compartments, said incubation compartments, said processing compartments are built as separate entities; furthermore, the distribution valve within the central distribution compartment comprises an essentially cylindrical valve cavity at one end of the distribution cavity and an essentially cylindrical valve core inserted into said valve cavity.
- the valve core is able to rotate within said valve cavity, and a multitude of flow channels which are provided in the valve core can establish different connections between said distribution cavity and any of the ducts leading to the distribution compartment's fitting surfaces by rotating the valve core.
- At least one incubation compartment comprises an incubation cavity constructed by a cylindrical shell, a plug arranged at the top end of the shell, and a multiway valve arranged at the bottom end of said shell, said plug comprises an air hole, said multiway valve is fitted with at least two fitting surfaces and provided with an essentially cylindrical valve cavity, and ducts to connect the valve cavity to the fitting surfaces and the incubation cavity.
- An essentially cylindrical valve core is inserted into said valve cavity and able to rotate in the valve cavity.
- At least two flow channels are provided in said valve core, said flow channels being able to connect the first or second fitting surface to said incubation cavity or the two fitting surfaces when rotating the valve core in the valve cavity.
- the design of the incubation compartment can be improved further if a sleeve is set at the outside of said shell, a cavity is formed between said sleeve and said shell, an exit and an entrance to said cavity are arranged at two opposite ends of said sleeve, a helical partition wall is provided in said cavity to form a helical channel surrounding said shell and connecting the exit and the entrance.
- the cavity between sleeve and shell can be used to control the incubators temperature by passing heating or cooling liquid through the cavity.
- An alternative solution to provide heating/cooling capability to the incubator is to use a helical duct surrounding said shell, characterized in that the inner diameter of said helical duct is slightly less than the outer diameter of the incubation cavity when the helical duct is not mounted on the shell.
- a processing compartment is provided with a duct and two electrodes. Those electrodes are arranged opposite to each other at both sides of the duct and electric couplers provided at the outer ends of said two electrodes can be used to connect an external power supply or a measurement amplifier.
- the electrodes can be separated by a non-conductive member for safety purposes and a flow guide can be grafted onto said member to guide the fluid flow between the electrodes.
- a processing compartment comprises a main duct and filter unit dividing said main duct into a front segment and a back segment.
- Said filter unit comprises a filter membrane and a porous support arranged at the back side of said filter membrane.
- the body of the processing compartment comprises a front part and a rear part which may be assembled into a whole body. A cavity for the membrane and porous support is formed between said front part and said rear part.
- a helical fluid guide is grafted into the front half part and connected to a duct leading to a third fitting surface for injecting external fluid between said filtration membrane and said front half part.
- An appropriate processing compartment is provided with an elongated filtration cavity connected at one end to a fitting surface via a duct.
- a choke plug is tightly fitted into said processing compartment at the other end of said filtration cavity.
- the choke plug has an internal duct and a fitting surface.
- a membrane filter tube inserted into said filtration cavity is attached to the inner end of said choke plug in such a way, that the duct is connected to the inside of the membrane filter tube.
- An additional duct connects a fitting surface at the side wall of the processing compartment with the filtration cavity, and said additional duct merges with the filtration cavity in tangential direction.
- the inner wall of the filtration cavity can be provided with a helical fluid guide.
- the fluid guide is connected to said additional port and arranged surrounding the membrane filter tube.
- a processing compartment is provided with a cavity and ducts that connect said cavity to two fitting surfaces.
- the processing compartment is provided with an optical pathway penetrating the cavity at an angle.
- the two ends of said optical pathway are formed by a light source and a light sensor respectively, said light source and light sensor are connected to the cavity by means of a transparent waveguide component.
- the optical pathway can be placed at an angle to the distribution cavity in the central distribution compartment. This will reduce the number of steps required to measure cell concentration as the concentration can be measured as soon as the cell suspension enters the distribution cavity.
- the benefit of the present invention is that a compact, flexible and automated assembly of different compartments offers to eliminate repetitive manual labor, shorten waiting and processing times, and reduce the possibility of human error and exposure to potentially harmful or dangerous agents.
- the modular design allows to run different kinds of processes and to combine systems to run several experiments in parallel.
- FIG. 1 shows a possible embodiment of the invention.
- FIG. 2 shows a possible embodiment of the central distribution valve.
- FIG. 3 shows the valve core of an embodiment of the central distribution valve rotated to position I
- FIG. 4 shows the valve core of an embodiment of the central distribution valve rotated to position II.
- FIG. 5 shows the valve core of an embodiment of the central distribution valve rotated to position III.
- FIG. 6 shows the valve core of an embodiment of the central distribution valve rotated to position III′.
- FIG. 7 shows the valve core of an embodiment of the central distribution valve rotated to position IV.
- FIG. 8 is the sectional view of the location A-A in the FIG. 1 .
- FIG. 9 is the sectional view of the location B-B in the FIG. 8 .
- FIG. 10 shows a second possible embodiment of the incubation compartments heating/cooling jacket.
- FIG. 11 shows a possible embodiment of the electrical processing compartment.
- FIG. 12 is the sectional view of the location C-C in the FIG. 11 .
- FIG. 13 shows a first possible embodiment of a filtration compartment.
- FIG. 14 is the sectional view of the location D-D in the FIG. 13 .
- FIG. 15 shows an exploded view of the filtration compartment's embodiment shown in FIG. 12 .
- FIG. 16 shows a second possible embodiment of the filtration compartment.
- FIG. 17 is the sectional view of the location E-E in the FIG. 16 .
- FIG. 18 shows a modification of the second possible embodiment of the filtration compartment.
- FIG. 19 shows a first possible embodiment of the cell density measurements compartment.
- FIG. 20 shows a second possible embodiment of the cell density measurements compartment.
- FIG. 21 illustrates the idea of using a common shape as the basis to design the different compartments.
- FIG. 22 shows a possible embodiment of a combined processing compartment with filtration and electrical processing capability
- FIG. 1 shows a simple embodiment of the invention as an example. It comprises of one central distribution compartment 1 , one incubation compartment 2 , and a single processing compartment 3 , for which—for the sake of this description—a simple filtration compartment is chosen as example.
- the central distribution compartment 1 Surrounding the central distribution valve 13 the central distribution compartment 1 provides three fitting surfaces capable of connecting to other compartments, in this case the incubation compartment 2 , the processing compartment 3 , and an external connector 243 .
- three ducts 14 lead from the central distribution valve 13 to the three fitting surfaces.
- the central distribution valve 13 comprises the valve cavity 131 arranged at one end of the distribution cavity 11 and the valve core 132 inserted into the bore 131 and capable of rotating within the valve cavity 131 .
- the valve cavity 131 and the valve core are mainly cylindrical in nature, but may have a tapered wall to reduce leakage between the walls of the valve cavity 131 and the valve core 132 .
- One or more flow channels 133 are provided inside the valve core 132 or on its surface in such a way that said channels 133 may connect the distribution cavity 11 with any of the ducts 14 when the valve core 132 is rotated.
- the flow channels 133 of the valve core 132 may have different shapes.
- a flow channel 133 may penetrate through the valve core 132 or it may be located at the surface of the valve core 132 .
- the valve core 132 shown in FIG. 1 uses a penetrating flow channel 133 to connect two locations on opposite sides of the valve cavity 131 and two flow channels at the surface of the valve core 132 to connect locations which are approximately at a 90 degree angle.
- the length of flow channels 133 may be chosen to adapt to angles other than 90 or 180 degrees.
- Two elastic seal elements 136 are arranged at the two sides of the flow channels 133 on the valve core 132 to prevent fluid leakage along the long axis of the valve core 132 .
- FIG. 3 to FIG. 7 show four operation positions of the central distribution valve 13 shown in FIG. 1 .
- the valve core 132 rotates to position I
- the incubation compartment 2 is connected to the distribution cavity 11
- the processing compartment 3 is connected to duct 14 therebelow which allows to transfer fluids from an external source through an external connector 243 .
- valve core 132 When the valve core 132 rotates to position IV, all of the ducts 14 and the distribution cavity 11 are separated from each other; this position may be used for the standby mode of the equipment.
- valve with slightly different characteristics can be obtained by varying the position, number, and length of the flow channels 133 and ducts 14 with respect to the distribution cavity 11 .
- the central distribution valve 13 is located directly at one end of the distribution cavity 11 , which reduces the residual fluid volume between the distribution cavity 11 and the distribution valve 13 to the minimum.
- An external connector 243 is mounted to the standard shape block 241 , and flow channels 244 which are provided on the valve core 242 allow to establish a connection between said external connector 243 and the duct 4 leading to the cultivation cavity. If air is blown into the device and lead from said connector 243 to the cultivation cavity 23 , the generated bubbles will provide oxygen for the cells within the cultivation cavity 23 and kinetic energy to agitate and blend the cell suspension in the cultivation cavity 23 . By rotating the valve core 242 , the flow channels 244 may also isolate the cultivation cavity 23 , or establish a connection between the cultivation cavity 23 and the central distribution valve.
- a sleeve 25 is set at the outside of the shell 21 , such that a cavity 26 is formed between the sleeve 25 and the shell 21 .
- An exit 251 and entrance 252 are connected to the cavity 26 and arranged at two opposite ends of the sleeve 25 . Cooling or heating fluid may be transported into the formed cavity 26 through the entrance 252 and returned to the heating/cooling system through the exit 251 .
- a helical partition wall is provided in the cavity 26 to form a helical channel surrounding the shell 21 and connecting the exit 251 and the entrance 252 to guide the fluid flow (not shown).
- FIG. 10 Another embodiment of heating or cooling the culture cavity 23 is shown in the FIG. 10 , wherein a helical duct 27 is provided surrounding the shell 21 , and the heating or cooling fluid runs in the helical duct 27 .
- the inner diameter of the helical duct is slightly less than the outer diameter of the sleeve 21 , thus the helical duct 27 clings to the shell 21 .
- it can be unwound slightly to increase its inner diameter.
- the advantage of this design is that the heating/cooling fluid remains well contained inside the helical duct 27 when said helical ducts is removed.
- processing compartments 3 are described, in particular, an electric processing compartment, two embodiments of a filtration compartment, and two embodiments of a cell density measurement compartment.
- FIGS. 11 and 12 shows an electric processing compartment comprising of a standard shape block 311 with ducts 4 which are accessible through fitting surfaces.
- Two electrodes 312 are inserted into the standard shape block 311 on opposite sides of the duct 4 , electric connectors 313 are provided at the outer ends of said two electrodes and are used to connect an external power supply or an electric measurement device.
- the standard shape block 311 is made from electrically insulating material, and allows exposing the cell suspension to AC voltage, DC voltage, or a transient voltage pulse.
- This interaction may be used for measuring the electric properties of the cell suspension between the electrodes or for altering the cell properties, for example a short transient current created by high voltage pulse may temporarily render cell membranes open for transport of plasmids or the oligonucleotides into the cell (electro-transformation).
- the power supply will be connected to electrodes 312 through the connectors 313 , a certain small volume of cell suspension will be transported into the cavity between the two electrodes 312 , and exposed to the voltage.
- the frequency of the electric shocks can be matched to the flow rate of the cell suspension to avoid over-exposure.
- an insulating member 314 is arranged between the two electrodes 312 , and a flow channel for guiding the fluid between the electrodes 312 is formed by said insulating member 314 .
- FIG. 13 , FIG. 14 and FIG. 15 show a first possible embodiment of a processing compartment with filtration capability.
- the filtration compartment is encapsulated in a standard shape block 321 and a main duct 4 connects the fitting surfaces with the membrane cavity.
- the membrane cavity contains a filter membrane 322 and a porous component 323 which divide the main duct into a front and a back segment.
- the standard shape block 321 comprises a front part 324 and a rear part 325 which may be assembled into a whole body, while a cavity for the filter membrane 322 and a porous component 323 is arranged between said front and rear parts. Changing the filter membrane 322 may be accomplished by means of detaching the front part 324 and the rear part 325 .
- a helical flow guide 326 is grafted into the front section 324 in such a way that it is in close proximity to the filter membrane 322 when the front 324 and rear 325 parts are joined together.
- the helical flow guide 326 is connected to a port 327 for injecting fluid from the side of the front part 324 .
- cell suspension first flows through the front part 324 until it reaches the filter membrane 322 , the liquid passes the filter membrane 322 and the porous component 323 , while the cells are deposited in the residue liquid on the surface of the filter membrane 322 in the helical flow guide 326 .
- the cells deposited on the surface of the filter membrane 322 may be re-suspended by means of two measures:
- port 327 is closed off, preferably by connecting a standard shape block with a valve to the fitting surface around port 327 . This makes sure that cell suspension will not escape through port 327 , but will be passed through the filter membrane 322 as described above.
- the cell suspension enters into the filtration cavity 332 from the side with the free end of the tubular filtration membrane 334 , and flows along the outside of the tubular filtration membrane 334 .
- the diameter of the filtration cavity 332 is slightly larger than the outer diameter of the tubular filtration membrane 334 , the volume between the filtration cavity 332 and the tubular filtration membrane 334 may be controlled to be very small.
- the cells are deposited at the outside surface of tubular filtration membrane 334 .
- the inner wall of the filtration cavity 332 can be lined with a helical flow guide 336 , which is connected to the port 335 and arranged surrounding the tubular filtration membrane 334 .
- Fresh fluid can thus flow through port 335 into the helical flow guide 336 which will impose and intensify a helical flow pattern of the liquid around the tubular filtration membrane 332 thus effectively lifting cells off the surface of the tubular filtration membrane 332 and re-suspending them in the fresh liquid.
- controlling the inner diameter of the second guide slot 336 can be used to reduce the residual fluid volume in the filtration compartment as much as possible.
- FIG. 19 shows a possible embodiment of a processing compartment with optical cell concentration measurement capability. It is contained in a standard shape block 341 provided with a duct 4 linking two fitting surfaces of the standard shape block 341 , which is provided with an optical channel penetrating the duct 4 at an angle, comprising a light source 343 , two light guides 344 on either side of the duct 4 , and a light sensor 342 .
- the light emitting from the light source 343 e.g. a light emitting diode, LED
- will travel through the first light guide 344 may interact with the cell suspension inside the duct 4 , enter the light guide 344 on the opposite side and then be received by the light sensor 342 (such as the photo-diode or photo-transistor).
- Cell density can then be estimated from the amount of light which has been extinguished through the interaction of light and cells in the suspension (as compared to a liquid without cells, e.g. using the Beer-Lambert-Equation).
- the cell concentration measurement can also be done in the central distribution compartment 1 , by arranging the optical channel as penetrating at an angle through the distribution cavity 11 .
- This design not only reduces the liquid volume required for the cell density measurement, but also reduces the need for mechanical movement.
- FIG. 21 illustrates this idea by using a common square shape 5 as the footprint of the “standard shape block” of all the compartments', in particular, the example shown in FIG. 21 combines two incubation compartments 2 with their multi-way valves, a central distribution compartment 1 , a single processing compartment 3 , and three additional multi-way valves.
- the footprint of all aforementioned compartments except the central distribution compartment 1 is one times the common square shape 5 , the central distribution compartment 1 has a footprint which is built from three common square shapes 5 .
- all compartments may be combined easily into different arrangements for different experimental designs.
- FIG. 22 shows a combined processing compartment.
- the aforesaid electric processing compartment and the filtration compartment with a flat filter membrane are combined in a standard shape block.
- the advantage of this combination is reducing the suspension volume of the duct 4 as more as possible, and meets the design of the common shape 5 .
- a groove 41 may be provided for a sealing element to prevent liquid leakage in the joint.
- compartments can be equipped with matching holes 43 in the fitting surface in such a way that alignment by means of the simple connector element 44 can be guaranteed, wherein the connector element 44 may be a simple cylindrical pin or a flat key.
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Abstract
The present invention discloses a device for cell culturing and processing, applicable in the field of biological and genetic engineering experiments, which comprises at least one central distribution compartment, at least one incubation compartment; at least one processing compartment, a number of ducts to transfer fluids between said compartments, wherein a distribution cavity and a piston capable of moving back and forth in said distribution cavity for altering the operational volume of said distribution cavity are provided within said central distribution compartment, and a distribution valve controlling the connection between said distribution cavity and said ducts is provided at one end of said distribution cavity within the distribution compartment.
During operation, cells grow and multiply in a cell suspension contained in the incubation compartment. The cell suspension may be transferred from said incubation compartment into one of the processing compartments by means of said central distribution valve and moving the piston within the distribution cavity. The present invention combines the central distribution compartments, the incubation compartments, and the processing compartments into a compact system, which replaces repetitive manual handling, saves time, avoids wasting raw experimental materials, reduces the risk of human exposure to hazardous materials, while accomplishing cell culturing and several types of cell processing experiments. The modular design and automatic operation allows running different types of experimental projects in a short amount of time, in particular experiments requiring multiple iterations.
Description
- The present invention describes a device used in the field of biological and genetic engineering, especially a device for cell cultivation, cell transformation and biological experiments.
- In the field of microbiology, especially in the field of biological engineering and genetic engineering, researchers have to verify their theories, ideas and designs by means of experiments on cell cultures. These experiments often include but are not limited to the following steps:
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- 1. Cell cultivation, especially making the cells grow and multiply in a liquid nutrient medium;
- 2. Measuring the cell concentration in the liquid nutrient medium;
- 3. Separating the cells from the liquid nutrient medium;
- 4. Resuspending the cells with fresh liquid.
- 5. Transforming cells by means of chemical, electrical, or other physical means, and by introducing genetic material such as plasmids or oligonucleotides, etc.;
- 6. Sterilizing the instruments with alcohol or other agents;
- 7. Rinsing the instruments with water.
- The current laboratory practice accomplishes the above steps through a sequence of manual operations on small batches of cells. The commonly used traditional experimental instruments include: test tube, shaker flask, shaking table, Petri dish, cuvette, syringe, pipette, centrifuge, membrane filter, and so on. When multiple rounds of experiments are required to achieve a desired result, considerable time and repetitive manual labor has to be invested in the process.
- Of course, it is possible to combine conventional equipment into small plants and add control systems to achieve some degree of automation. The main drawback of this approach is that the different components are usually not meant to be combined and do not have matching specifications. The resulting bio-chemical plant will be too big and the required volume of cell culture will be too large for convenient use in a laboratory or with expensive materials.
- In order to solve the above problem, the present invention provides a compact, flexible and automated device for cell culturing and processing, which, may be used for different experimental projects, substitute repetitive manual handling, save time and labor, avoid wasting of raw materials, and minimize the risk of human exposure to potentially dangerous substances.
- The technical solution for solving the above problem by the present invention is a device for cell culturing and processing, comprising at least one central distribution compartment, at least one incubation compartment; at least one processing compartment, a number of ducts to transfer fluids between said compartments, wherein a distribution cavity and a piston capable of moving back and forth in said distribution cavity for altering the operational volume of said distribution cavity are provided within said central distribution compartment, and a distribution valve controlling the connection between said distribution cavity and said ducts is provided at one end of said distribution cavity within the distribution compartment.
- During operation, the cells grow and multiply in the incubation compartment. After connecting the incubation compartment to the distribution cavity by choosing a suitable position of the distribution valve in the central distribution compartment, liquid can be transferred between the compartments by moving the piston within the distribution cavity. Likewise, the distribution cavity can be connected to any of the processing compartments, which offer the possibility to accomplish tasks including removing cells from the nutrition medium and re-suspending them in another liquid, cooling, heating, optical density measurement, conductivity measurement, electro-transformation, and exposure to electro-magnetic radiation.
- As a furthermore improvement of the technical solution of the present invention is that said central distribution compartments, said incubation compartments, said processing compartments are built as separate entities; furthermore, the distribution valve within the central distribution compartment comprises an essentially cylindrical valve cavity at one end of the distribution cavity and an essentially cylindrical valve core inserted into said valve cavity. The valve core is able to rotate within said valve cavity, and a multitude of flow channels which are provided in the valve core can establish different connections between said distribution cavity and any of the ducts leading to the distribution compartment's fitting surfaces by rotating the valve core.
- As a furthermore improvement of the technical solution of the present invention we consider that at least one incubation compartment comprises an incubation cavity constructed by a cylindrical shell, a plug arranged at the top end of the shell, and a multiway valve arranged at the bottom end of said shell, said plug comprises an air hole, said multiway valve is fitted with at least two fitting surfaces and provided with an essentially cylindrical valve cavity, and ducts to connect the valve cavity to the fitting surfaces and the incubation cavity. An essentially cylindrical valve core is inserted into said valve cavity and able to rotate in the valve cavity. At least two flow channels are provided in said valve core, said flow channels being able to connect the first or second fitting surface to said incubation cavity or the two fitting surfaces when rotating the valve core in the valve cavity.
- The design of the incubation compartment can be improved further if a sleeve is set at the outside of said shell, a cavity is formed between said sleeve and said shell, an exit and an entrance to said cavity are arranged at two opposite ends of said sleeve, a helical partition wall is provided in said cavity to form a helical channel surrounding said shell and connecting the exit and the entrance. The cavity between sleeve and shell can be used to control the incubators temperature by passing heating or cooling liquid through the cavity.
- An alternative solution to provide heating/cooling capability to the incubator is to use a helical duct surrounding said shell, characterized in that the inner diameter of said helical duct is slightly less than the outer diameter of the incubation cavity when the helical duct is not mounted on the shell.
- To add the ability to interact with cell suspension by means of electrical currents or voltages to the present invention, a processing compartment is provided with a duct and two electrodes. Those electrodes are arranged opposite to each other at both sides of the duct and electric couplers provided at the outer ends of said two electrodes can be used to connect an external power supply or a measurement amplifier. The electrodes can be separated by a non-conductive member for safety purposes and a flow guide can be grafted onto said member to guide the fluid flow between the electrodes.
- To add the ability to separate cells from the medium and to re-suspend cells in fresh medium, a processing compartment comprises a main duct and filter unit dividing said main duct into a front segment and a back segment. Said filter unit comprises a filter membrane and a porous support arranged at the back side of said filter membrane. The body of the processing compartment comprises a front part and a rear part which may be assembled into a whole body. A cavity for the membrane and porous support is formed between said front part and said rear part. On the front side of the filter membrane, a helical fluid guide is grafted into the front half part and connected to a duct leading to a third fitting surface for injecting external fluid between said filtration membrane and said front half part.
- Another possibility to provide filtration and re-suspension capability is to use a filter tube instead of a flat membrane. An appropriate processing compartment is provided with an elongated filtration cavity connected at one end to a fitting surface via a duct. A choke plug is tightly fitted into said processing compartment at the other end of said filtration cavity. The choke plug has an internal duct and a fitting surface. A membrane filter tube inserted into said filtration cavity is attached to the inner end of said choke plug in such a way, that the duct is connected to the inside of the membrane filter tube. An additional duct connects a fitting surface at the side wall of the processing compartment with the filtration cavity, and said additional duct merges with the filtration cavity in tangential direction.
- To improve re-suspension of cells from the membrane filter tube, the inner wall of the filtration cavity can be provided with a helical fluid guide. On one end, the fluid guide is connected to said additional port and arranged surrounding the membrane filter tube.
- To add the ability to measure cell concentration, a processing compartment is provided with a cavity and ducts that connect said cavity to two fitting surfaces. The processing compartment is provided with an optical pathway penetrating the cavity at an angle. The two ends of said optical pathway are formed by a light source and a light sensor respectively, said light source and light sensor are connected to the cavity by means of a transparent waveguide component.
- Instead of using a separate entity for cell concentration measurement, the optical pathway can be placed at an angle to the distribution cavity in the central distribution compartment. This will reduce the number of steps required to measure cell concentration as the concentration can be measured as soon as the cell suspension enters the distribution cavity.
- The benefit of the present invention is that a compact, flexible and automated assembly of different compartments offers to eliminate repetitive manual labor, shorten waiting and processing times, and reduce the possibility of human error and exposure to potentially harmful or dangerous agents. In addition the modular design allows to run different kinds of processes and to combine systems to run several experiments in parallel.
- The present invention will be further described below with reference to the drawings.
-
FIG. 1 shows a possible embodiment of the invention. -
FIG. 2 shows a possible embodiment of the central distribution valve. -
FIG. 3 shows the valve core of an embodiment of the central distribution valve rotated to position I -
FIG. 4 shows the valve core of an embodiment of the central distribution valve rotated to position II. -
FIG. 5 shows the valve core of an embodiment of the central distribution valve rotated to position III. -
FIG. 6 shows the valve core of an embodiment of the central distribution valve rotated to position III′. -
FIG. 7 shows the valve core of an embodiment of the central distribution valve rotated to position IV. -
FIG. 8 is the sectional view of the location A-A in theFIG. 1 . -
FIG. 9 is the sectional view of the location B-B in theFIG. 8 . -
FIG. 10 shows a second possible embodiment of the incubation compartments heating/cooling jacket. -
FIG. 11 shows a possible embodiment of the electrical processing compartment. -
FIG. 12 is the sectional view of the location C-C in theFIG. 11 . -
FIG. 13 shows a first possible embodiment of a filtration compartment. -
FIG. 14 is the sectional view of the location D-D in theFIG. 13 . -
FIG. 15 shows an exploded view of the filtration compartment's embodiment shown inFIG. 12 . -
FIG. 16 shows a second possible embodiment of the filtration compartment. -
FIG. 17 is the sectional view of the location E-E in theFIG. 16 . -
FIG. 18 shows a modification of the second possible embodiment of the filtration compartment. -
FIG. 19 shows a first possible embodiment of the cell density measurements compartment. -
FIG. 20 shows a second possible embodiment of the cell density measurements compartment. -
FIG. 21 illustrates the idea of using a common shape as the basis to design the different compartments. -
FIG. 22 shows a possible embodiment of a combined processing compartment with filtration and electrical processing capability - Referring to the
FIG. 1 toFIG. 22 , the present invention describes a device for cell cultivation and bioengineering experiments, comprising acentral distribution compartment 1, at least one incubation compartment 2, at least oneprocessing compartment 3, a plurality ofducts 4 to accomplish fluid transfer between said compartments, wherein, apiston 12 is capable of moving back and forth in adistribution cavity 11 of thecentral distribution compartment 1 for changing the operation volume of saiddistribution cavity 11, acentral distribution valve 13 is used to control the connection between saiddistribution cavity 11 and any one of saidducts 4, and saidcentral distribution valve 13 is located at one end of thedistribution cavity 11 within saidcentral distribution compartment 1. - Refer to the
FIG. 1 which shows a simple embodiment of the invention as an example. It comprises of onecentral distribution compartment 1, one incubation compartment 2, and asingle processing compartment 3, for which—for the sake of this description—a simple filtration compartment is chosen as example. Surrounding thecentral distribution valve 13 thecentral distribution compartment 1 provides three fitting surfaces capable of connecting to other compartments, in this case the incubation compartment 2, theprocessing compartment 3, and anexternal connector 243. Inside thecentral distribution compartment 1, threeducts 14 lead from thecentral distribution valve 13 to the three fitting surfaces. Thecentral distribution valve 13 comprises thevalve cavity 131 arranged at one end of thedistribution cavity 11 and thevalve core 132 inserted into thebore 131 and capable of rotating within thevalve cavity 131. Thevalve cavity 131 and the valve core are mainly cylindrical in nature, but may have a tapered wall to reduce leakage between the walls of thevalve cavity 131 and thevalve core 132. One ormore flow channels 133 are provided inside thevalve core 132 or on its surface in such a way that saidchannels 133 may connect thedistribution cavity 11 with any of theducts 14 when thevalve core 132 is rotated. - As shown in
FIG. 2 , one end of thevalve core 132 of thedistribution valve 13 is provided with aprotuberance 134 on one end and a fixation element 135 (such as a Seeger snap ring or a disc spring) on the other end which are used to fix thevalve core 132 in the correct axial position inside thevalve cavity 131. Obviously, afixation element 135 may also replace theprotuberance 134 to define the axial position of thevalve core 132 inside thevalve cavity 131. - The
flow channels 133 of thevalve core 132 may have different shapes. For example, aflow channel 133 may penetrate through thevalve core 132 or it may be located at the surface of thevalve core 132. Thevalve core 132 shown inFIG. 1 uses a penetratingflow channel 133 to connect two locations on opposite sides of thevalve cavity 131 and two flow channels at the surface of thevalve core 132 to connect locations which are approximately at a 90 degree angle. By adjustment, the length offlow channels 133 may be chosen to adapt to angles other than 90 or 180 degrees. - Two
elastic seal elements 136 are arranged at the two sides of theflow channels 133 on thevalve core 132 to prevent fluid leakage along the long axis of thevalve core 132. - The
FIG. 3 toFIG. 7 show four operation positions of thecentral distribution valve 13 shown inFIG. 1 . When thevalve core 132 rotates to position I, the incubation compartment 2 is connected to thedistribution cavity 11, and theprocessing compartment 3 is connected toduct 14 therebelow which allows to transfer fluids from an external source through anexternal connector 243. - When the
valve core 132 rotates to position II, thedistribution cavity 11 is connected to saidprocessing compartment 3, while theducts 14 thereabove and therebelow are closed off. - When the
valve core 132 rotates to position III, the incubation compartment 2 and theprocessing compartment 3 are connected, while thedistribution cavity 11 is connected to theduct 14 therebelow (e.g. to draw fluids from an external source into the distribution cavity 11). It should be noted that, in position III, in order to prevent the connection of the incubation compartment 2 and theprocessing compartment 3, the position may be changed by a few degrees from position III to position III′. Because the diameters of thedistribution cavity 11 and theducts 14 are different, thedistribution cavity 11 may remain connected to theduct 14 therebelow, while keeping theother ducts 14 closed off. - When the
valve core 132 rotates to position IV, all of theducts 14 and thedistribution cavity 11 are separated from each other; this position may be used for the standby mode of the equipment. - It is obvious to those skilled in the art that, the valve with slightly different characteristics can be obtained by varying the position, number, and length of the
flow channels 133 andducts 14 with respect to thedistribution cavity 11. - In the present invention, the
piston 12 is inserted into thedistribution cavity 11 within thecentral distribution compartment 1 and may move axially in saiddistribution cavity 11. Thepiston 12 comprises of arigid member 121 connected to a linear actuating device (not shown) and aflexible member 122 attached to the front end of saidrigid member 121. This type of design is known from medical syringes and the syringe pump, and to use the design for the present invention possessed the following three advantages: -
- (i) The motion of
piston 12 and itsflexible member 122 along the walls of thedistribution cavity 11 can keep the inner wall of saiddistribution cavity 11 clean. The self-cleaning function eliminates the need for additional cleaning steps and allows to use the samecentral distribution compartment 1 for different kinds of media; - (ii) The motion of
piston 12 and itsflexible member 122 along the walls of thedistribution cavity 11 can be used to draw and push liquids of different viscosity, solid-liquid suspensions (such as cell suspensions), and gases; - (iii) By using the cross-sectional area of the
distribution cavity 11, the linear motion ofpiston 12 can be easily used to calculate dispensed volumes or volumetric flow rates. If the driving force from the linear actuator is known, the system pressure can be calculated as well.
- (i) The motion of
- In addition, the
central distribution valve 13 is located directly at one end of thedistribution cavity 11, which reduces the residual fluid volume between thedistribution cavity 11 and thedistribution valve 13 to the minimum. - Refer to the
FIG. 8 andFIG. 9 , the incubation compartment 2 comprises acultivation cavity 23 constructed by acylindrical shell 21 and aplug 22 arranged at the top end of theshell 21 and amultiway valve 24 arranged at the bottom-end of the shell. Theplug 22 comprises anair hole 221 and seals theshell 21 with anelastic sealing element 222. Themultiway valve 24 adopts a similar design to thecentral distribution valve 13, and is fitted into astandard shape block 241, said standard shape block being able to connect to other compartments through the provided fitting surfaces. As thecentral distribution valve 13, themulti-way valve 24 has a valve cavity, a plurality of ducts, and avalve core 242 inserted into said valve cavity and capable of rotating in said valve cavity. Anexternal connector 243 is mounted to thestandard shape block 241, and flowchannels 244 which are provided on thevalve core 242 allow to establish a connection between saidexternal connector 243 and theduct 4 leading to the cultivation cavity. If air is blown into the device and lead from saidconnector 243 to thecultivation cavity 23, the generated bubbles will provide oxygen for the cells within thecultivation cavity 23 and kinetic energy to agitate and blend the cell suspension in thecultivation cavity 23. By rotating thevalve core 242, theflow channels 244 may also isolate thecultivation cavity 23, or establish a connection between thecultivation cavity 23 and the central distribution valve. - In one embodiment of the invention, a
sleeve 25 is set at the outside of theshell 21, such that acavity 26 is formed between thesleeve 25 and theshell 21. Anexit 251 andentrance 252 are connected to thecavity 26 and arranged at two opposite ends of thesleeve 25. Cooling or heating fluid may be transported into the formedcavity 26 through theentrance 252 and returned to the heating/cooling system through theexit 251. In order to improve the heat conduction, a helical partition wall is provided in thecavity 26 to form a helical channel surrounding theshell 21 and connecting theexit 251 and theentrance 252 to guide the fluid flow (not shown). - Another embodiment of heating or cooling the
culture cavity 23 is shown in theFIG. 10 , wherein ahelical duct 27 is provided surrounding theshell 21, and the heating or cooling fluid runs in thehelical duct 27. The inner diameter of the helical duct is slightly less than the outer diameter of thesleeve 21, thus thehelical duct 27 clings to theshell 21. When it is necessary to remove theduct 27, it can be unwound slightly to increase its inner diameter. The advantage of this design is that the heating/cooling fluid remains well contained inside thehelical duct 27 when said helical ducts is removed. - In the following, several embodiments of
possible processing compartments 3 are described, in particular, an electric processing compartment, two embodiments of a filtration compartment, and two embodiments of a cell density measurement compartment. -
FIGS. 11 and 12 shows an electric processing compartment comprising of astandard shape block 311 withducts 4 which are accessible through fitting surfaces. Twoelectrodes 312 are inserted into thestandard shape block 311 on opposite sides of theduct 4,electric connectors 313 are provided at the outer ends of said two electrodes and are used to connect an external power supply or an electric measurement device. Specifically, thestandard shape block 311 is made from electrically insulating material, and allows exposing the cell suspension to AC voltage, DC voltage, or a transient voltage pulse. This interaction may be used for measuring the electric properties of the cell suspension between the electrodes or for altering the cell properties, for example a short transient current created by high voltage pulse may temporarily render cell membranes open for transport of plasmids or the oligonucleotides into the cell (electro-transformation). During operation, the power supply will be connected toelectrodes 312 through theconnectors 313, a certain small volume of cell suspension will be transported into the cavity between the twoelectrodes 312, and exposed to the voltage. The frequency of the electric shocks can be matched to the flow rate of the cell suspension to avoid over-exposure. To avoid the accidental contact of the twoelectrodes 312, an insulatingmember 314 is arranged between the twoelectrodes 312, and a flow channel for guiding the fluid between theelectrodes 312 is formed by said insulatingmember 314. -
FIG. 13 ,FIG. 14 andFIG. 15 show a first possible embodiment of a processing compartment with filtration capability. The filtration compartment is encapsulated in astandard shape block 321 and amain duct 4 connects the fitting surfaces with the membrane cavity. The membrane cavity contains afilter membrane 322 and aporous component 323 which divide the main duct into a front and a back segment. Thestandard shape block 321 comprises afront part 324 and arear part 325 which may be assembled into a whole body, while a cavity for thefilter membrane 322 and aporous component 323 is arranged between said front and rear parts. Changing thefilter membrane 322 may be accomplished by means of detaching thefront part 324 and therear part 325. Ahelical flow guide 326 is grafted into thefront section 324 in such a way that it is in close proximity to thefilter membrane 322 when the front 324 and rear 325 parts are joined together. Thehelical flow guide 326 is connected to aport 327 for injecting fluid from the side of thefront part 324. During operation, cell suspension first flows through thefront part 324 until it reaches thefilter membrane 322, the liquid passes thefilter membrane 322 and theporous component 323, while the cells are deposited in the residue liquid on the surface of thefilter membrane 322 in thehelical flow guide 326. After filtering, the cells deposited on the surface of thefilter membrane 322 may be re-suspended by means of two measures: -
- (i) Fresh fluid may be introduced through the
rear part 325 and pressed through thefilter membrane 322 from the back side of thefilter membrane 322; - (ii) Fresh fluid may be injected into the
front part 324 through theport 327 and thehelical flow guide 326 which causes the fresh fluid to flow over the cells deposited on thefilter membrane 322.
- (i) Fresh fluid may be introduced through the
- While cells are being deposited on the
filtration membrane 322 at the beginning of the process,port 327 is closed off, preferably by connecting a standard shape block with a valve to the fitting surface aroundport 327. This makes sure that cell suspension will not escape throughport 327, but will be passed through thefilter membrane 322 as described above. -
FIG. 16 andFIG. 17 show a second possible embodiment of afiltration compartment 331 whose outer dimensions are equivalent to the combined size of several standard shape blocks. Thefiltration compartment 331 provides afiltration cavity 332 which is connected to a fitting surface by aduct 4. Inside the filtration cavity, afilter membrane tube 334 is placed. Achoke plug 333 with aninternal duct 4 and a tubular membrane filter arranged on a cylinder shaped protuberance on the inner side of thechoke plug 333 and joint tightly to thechoke plug 333 with resin, is inserted into the filtration compartment at the other end of the filtration cavity. Once inserted, thechoke plug 333 constitutes one end of thefiltration cavity 332 and is sealed against the housing of the compartment by an elastic sealing element. During operation, the cell suspension enters into thefiltration cavity 332 from the side with the free end of thetubular filtration membrane 334, and flows along the outside of thetubular filtration membrane 334. By designing the diameter of thefiltration cavity 332 to be slightly larger than the outer diameter of thetubular filtration membrane 334, the volume between thefiltration cavity 332 and thetubular filtration membrane 334 may be controlled to be very small. While the liquid passes through thetubular filtration membrane 334 and theduct 4 in thechoke plug 333, the cells are deposited at the outside surface oftubular filtration membrane 334. For this second embodiment of the filtration compartment, there are two methods to re-suspend the cells deposited on the outside of the tubular filtration membrane: -
- (1) Fresh fluid may be introduced through the
duct 4 in thechoke plug 333 and pressed to penetrate reversely through thetubular filtration membrane 334; - (2) Fresh fluid may enter into the
filtration cavity 332 from theport 335, to generate a helical flow pattern around thetubular filtration membrane 334 which will lift the deposited cells off the surface of thetubular filtration membrane 334.
- (1) Fresh fluid may be introduced through the
- Refer to the
FIG. 18 , as a further improvement of the second embodiment, the inner wall of thefiltration cavity 332 can be lined with ahelical flow guide 336, which is connected to theport 335 and arranged surrounding thetubular filtration membrane 334. Fresh fluid can thus flow throughport 335 into thehelical flow guide 336 which will impose and intensify a helical flow pattern of the liquid around thetubular filtration membrane 332 thus effectively lifting cells off the surface of thetubular filtration membrane 332 and re-suspending them in the fresh liquid. Similarly, controlling the inner diameter of thesecond guide slot 336 can be used to reduce the residual fluid volume in the filtration compartment as much as possible. -
FIG. 19 shows a possible embodiment of a processing compartment with optical cell concentration measurement capability. It is contained in astandard shape block 341 provided with aduct 4 linking two fitting surfaces of thestandard shape block 341, which is provided with an optical channel penetrating theduct 4 at an angle, comprising alight source 343, twolight guides 344 on either side of theduct 4, and alight sensor 342. The light emitting from the light source 343 (e.g. a light emitting diode, LED), will travel through thefirst light guide 344, may interact with the cell suspension inside theduct 4, enter thelight guide 344 on the opposite side and then be received by the light sensor 342 (such as the photo-diode or photo-transistor). Cell density can then be estimated from the amount of light which has been extinguished through the interaction of light and cells in the suspension (as compared to a liquid without cells, e.g. using the Beer-Lambert-Equation). - As shown in the
FIG. 20 , the cell concentration measurement can also be done in thecentral distribution compartment 1, by arranging the optical channel as penetrating at an angle through thedistribution cavity 11. This design not only reduces the liquid volume required for the cell density measurement, but also reduces the need for mechanical movement. Once the connection from the incubation compartment 2 to thecentral distribution compartment 1 has been established, cell concentration can be measured as soon as the cell suspension reaches to thecavity 11. Furthermore, on account of the greater diameter of thedistribution cavity 11, a more accurate measurement can be performed along the longer optical path through the cell suspension. - In order to allow experimenters to arrange the compartments freely according to their experimental design, the present invention adopts the idea of a “standard shape block” as the basis of all compartments.
FIG. 21 illustrates this idea by using a common square shape 5 as the footprint of the “standard shape block” of all the compartments', in particular, the example shown inFIG. 21 combines two incubation compartments 2 with their multi-way valves, acentral distribution compartment 1, asingle processing compartment 3, and three additional multi-way valves. The footprint of all aforementioned compartments except thecentral distribution compartment 1 is one times the common square shape 5, thecentral distribution compartment 1 has a footprint which is built from three common square shapes 5. Thus all compartments may be combined easily into different arrangements for different experimental designs. - The
FIG. 22 shows a combined processing compartment. The aforesaid electric processing compartment and the filtration compartment with a flat filter membrane are combined in a standard shape block. The advantage of this combination is reducing the suspension volume of theduct 4 as more as possible, and meets the design of the common shape 5. - Refer to the
FIG. 1 , in order to connect the two adjacent compartments, the external exits of theducts 4 of the different compartments will align with each other the boundaries of the compartments are aligned. Around each exit of theducts 4, agroove 41 may be provided for a sealing element to prevent liquid leakage in the joint. - In order to ensure good alignment of two adjacent compartments, compartments can be equipped with matching holes 43 in the fitting surface in such a way that alignment by means of the simple connector element 44 can be guaranteed, wherein the connector element 44 may be a simple cylindrical pin or a flat key.
- Certainly, the present invention is not limited to the above embodiments, the skilled person in the field may think of equivalent modifications or alternatives in the premise of not prejudice to the which are also in agreement with the spirit of the present invention, and these equivalent modifications or alternatives are all be comprised in the scope defined by the claims of this application.
Claims (11)
1. A device for cell culturing and processing, which comprises at least one central distribution compartment, at least one incubation compartment; at least one processing compartment, a number of ducts to transfer fluids between said compartments, wherein a distribution cavity and a piston capable of moving back and forth in said distribution cavity for altering the operational volume of said distribution cavity are provided within said central distribution compartment, and a distribution valve controlling the connection between said distribution cavity and said ducts is provided at one end of said distribution cavity within the distribution compartment.
2. The device for cell culturing and processing of claim 1 , characterized in that, said central distribution compartments, said incubation compartments, said processing compartments are built as separate entities, in such a way that each entity's body is equivalent to one or more standard shape blocks, ducts in said entities are connected to a number of fitting surfaces on said entities, said entities can be joined together at the fitting surfaces to connect the ducts in said entities, said distribution valve within the distribution compartment comprises an essentially cylindrical valve cavity at one end of the distribution cavity and an essentially cylindrical valve core inserted into said valve cavity, where the valve core is able to rotate within said valve cavity, and a multitude of flow channels provided in the valve core can establish different connections between said distribution cavity and any of the ducts leading to the distribution compartment's fitting surfaces by rotating the valve core.
3. The device for cell culturing and processing of claim 2 , characterized in that at least one incubation compartment comprises an incubation cavity constructed by a cylindrical shell, a plug arranged at the top end of the shell, and a multiway valve arranged at the bottom end of said shell, said plug comprises an air hole, said multiway valve is fitted in a body the volume of which is equivalent to one or more standard shape blocks and said body having at least two fitting surfaces and provided with an essentially cylindrical valve cavity, ducts to connect said valve cavity to the fitting surfaces and the incubation cavity, an essentially cylindrical valve core inserted into said valve cavity and able to rotate in the valve cavity, at least two flow channels are provided in said valve core, said flow channels being able to connect the first fitting surface to said incubation cavity, to connect the second fitting surface to the said incubation cavity, or to connect the two fitting surfaces when rotating the valve core in the valve cavity.
4. The device for cell culturing and processing of claim 3 , characterized in that, a sleeve is set at the outside of said shell, a cavity is formed between said sleeve and said shell, an exit and an entrance to said cavity are arranged at two opposite ends of said sleeve, a helical partition wall is provided in said cavity to form a helical channel surrounding said shell and connecting the exit and the entrance.
5. The device for cell culturing and processing of claim 3 , characterized in that, a helical duct is provided surrounding said shell, characterized in that the inner diameter of said helical duct is slightly less than the outer diameter of the incubation cavity when the helical duct is not mounted on the shell, and that the tension created by expanding the helical duct when fitting it on said shell will provide intimate contact between said helical duct and said shell.
6. The device for cell culturing and processing of claim 2 , characterized in that one of said processing units is housed in a body the volume of which is equivalent to one or more standard shape blocks, said body is provided with two ducts which connect two fitting surfaces to a central cavity, characterized in that two electrodes are arranged opposite to each other at each sides of said cavity, electric connectors are provided to connect an external power supply or an electrical measurement amplifier at the outer ends of said two electrodes, an insulation member is arranged inside the cavity between the two electrodes, and a flow channel is formed on said insulation member to guide the liquid flow through said cavity between said two electrodes.
7. The device for cell culturing and processing of claim 2 , characterized in that, one of said processing compartments is housed in a body the volume of which is equivalent to one or more standard shape blocks, said body is provided with a main duct connected to two of the body's fitting surfaces, and a filter unit dividing the main duct into a front segment and a back segment, said filter unit comprises a filter membrane and a porous support arranged at the back side of said filter membrane, said body comprises a front part and a rear part which may be assembled into a whole body, a cavity for the membrane and porous support is formed between said front part and said rear part, a helical fluid guide is provided in close proximity to said filter membrane in said front part, said helical flow guide is connected to a side duct leading to a third fitting surface for injecting external fluid between said filtration membrane and said front part.
8. The device for cell culturing and processing of claim 2 , characterized in that, one of said processing compartments is housed in a body the volume of which is equivalent to one or more standard shape blocks, in its interior said body is provided with a filtration cavity extending essentially along the long axis of said body, one end of said filtration cavity is connected to a fitting surface by means of a duct, a choke plug is tightly fitted into said processing compartment at the other end of said filtration cavity and provided with an internal duct and a fitting surface, a membrane filter tube inserted into said filtration cavity is attached to the inner end of said choke plug so that said internal duct connects the inside of the filter tube to said fitting surface of said choke plug, and an additional duct connects the filtration cavity with a third fitting surface at the side wall of the processing compartment, and said additional duct merges with the filtration cavity in tangential direction.
9. The device for cell culturing and processing of claim 8 , characterized in that, the inner wall of the filtration cavity is provided with a helical fluid guide, which is connected to said additional duct and third fitting surface and arranged surrounding the membrane filter tube inside the filtration cavity.
10. The device for cell culturing and processing of claim 2 , characterized in that one of said processing units is housed in a body the volume of which is equivalent to one or more standard shape blocks, said body is provided with ducts which connect two fitting surfaces to a cavity, an optical pathway penetrating the cavity at an angle, the two ends of said optical pathway are formed by a light source and a light sensor respectively, light source and light sensor are connected to the cavity by means of a transparent waveguide component.
11. The device for cell culturing and processing of claim 1 , characterized in that, said central distribution compartment is provided with an optical pathway penetrating the distribution cavity at an angle, the two ends of said optical pathway are formed by a light source and a light sensor respectively, light source and light sensor are connected to the distribution cavity by means of a transparent waveguide component.
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN201410112722.6 | 2014-03-25 | ||
| CN201410112722.6A CN103881911B (en) | 2014-03-25 | 2014-03-25 | A kind of cell culture and experimental device |
| PCT/CN2014/075210 WO2015143743A1 (en) | 2014-03-25 | 2014-04-11 | Apparatus for cell culture and experiment |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| US20170130183A1 true US20170130183A1 (en) | 2017-05-11 |
Family
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| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| US14/434,661 Abandoned US20170130183A1 (en) | 2014-03-25 | 2014-04-11 | Device for Cell Culturing and Processing |
| US15/275,503 Active 2035-02-02 US10407656B2 (en) | 2014-03-25 | 2016-09-26 | Cell culture and experiment device |
Family Applications After (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| US15/275,503 Active 2035-02-02 US10407656B2 (en) | 2014-03-25 | 2016-09-26 | Cell culture and experiment device |
Country Status (4)
| Country | Link |
|---|---|
| US (2) | US20170130183A1 (en) |
| EP (1) | EP3124595B1 (en) |
| CN (1) | CN103881911B (en) |
| WO (1) | WO2015143743A1 (en) |
Cited By (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US10407656B2 (en) * | 2014-03-25 | 2019-09-10 | Guangzhou Institute Of Advanced Technology, Chinese Academy Of Sciences | Cell culture and experiment device |
Families Citing this family (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| DE102017125881B4 (en) * | 2017-11-06 | 2019-06-19 | Sartorius Stedim Biotech Gmbh | Filter module and method for detecting microorganisms |
| CN109777733B (en) * | 2019-02-26 | 2022-02-01 | 中国人民解放军军事科学院军事医学研究院 | Microwave biological effect irradiation device |
| CN112625900B (en) * | 2020-12-17 | 2022-05-17 | 西安电子科技大学 | Experimental device for electromagnetic irradiation of cells with tilted waveguide resonator |
| CN114672415B (en) * | 2022-04-08 | 2022-12-20 | 湖北明德健康科技有限公司 | Diluting device |
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| PT2204440T (en) * | 1998-02-19 | 2016-10-18 | Medical Electronic Systems Llc | Sperm analysis system |
| US6374684B1 (en) * | 2000-08-25 | 2002-04-23 | Cepheid | Fluid control and processing system |
| ES2208127B1 (en) * | 2002-11-28 | 2005-09-01 | Universitat Politecnica De Catalunya | MODULAR SYSTEM OF MULTIPLES AUTOMATED MINIBIOR REACTORS FOR MULTIFUNCTIONAL SCREENNING (HTS) IN BIOTECHNOLOGY. |
| US8876765B2 (en) * | 2007-05-16 | 2014-11-04 | Smiths Medical Asd, Inc. | Pump module for use in a medical fluid dispensing system |
| WO2010016800A1 (en) * | 2008-08-08 | 2010-02-11 | Agency For Science, Technology And Research | Microfluidic continuous flow device |
| DK2382514T3 (en) * | 2008-12-23 | 2019-02-04 | Xoma Us Llc | Flexible production system |
| US9090863B2 (en) * | 2010-05-17 | 2015-07-28 | Pall Corporation | System for seeding cells onto three dimensional scaffolds |
| EP2604679B1 (en) * | 2011-01-17 | 2016-09-28 | Tokyo Women's Medical University | Cell culture treatment system, and method for connection of modules for cell culture treatment system |
| CN103881911B (en) * | 2014-03-25 | 2015-09-09 | 广州中国科学院先进技术研究所 | A kind of cell culture and experimental device |
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2014
- 2014-03-25 CN CN201410112722.6A patent/CN103881911B/en active Active
- 2014-04-11 US US14/434,661 patent/US20170130183A1/en not_active Abandoned
- 2014-04-11 WO PCT/CN2014/075210 patent/WO2015143743A1/en not_active Ceased
- 2014-04-11 EP EP14887546.1A patent/EP3124595B1/en not_active Not-in-force
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2016
- 2016-09-26 US US15/275,503 patent/US10407656B2/en active Active
Patent Citations (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US20050175273A1 (en) * | 2002-08-02 | 2005-08-11 | Kazuhiro Iida | Microchip, method of manufacturing microchip, and method of detecting compositions |
| US20080038737A1 (en) * | 2006-05-01 | 2008-02-14 | Cepheid | Methods and apparatus for sequential amplification reactions |
| US20080026451A1 (en) * | 2006-06-15 | 2008-01-31 | Braman Jeffrey C | System for isolating biomolecules from a sample |
Cited By (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US10407656B2 (en) * | 2014-03-25 | 2019-09-10 | Guangzhou Institute Of Advanced Technology, Chinese Academy Of Sciences | Cell culture and experiment device |
Also Published As
| Publication number | Publication date |
|---|---|
| CN103881911B (en) | 2015-09-09 |
| CN103881911A (en) | 2014-06-25 |
| EP3124595A1 (en) | 2017-02-01 |
| US20170009196A1 (en) | 2017-01-12 |
| EP3124595A4 (en) | 2017-11-15 |
| EP3124595B1 (en) | 2020-04-22 |
| WO2015143743A1 (en) | 2015-10-01 |
| US10407656B2 (en) | 2019-09-10 |
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