Patent Application
20250010287
The present invention relates to an integrated chip that has an integrated function capable of providing cell image and biochemical detection, and more particularly relates to a microfluidic biological detection chip that includes a cell fluid chamber and an electrochemistry detection area.
Biochemical characteristic analysis and the image for a specific cell is generally applied in biomedical detection and can provide qualitative and quantitative research for cell and molecule target and medical efficacy evaluation related, etc.
A microfluidic chip can be used for detecting microparticles, such as cells, genetic materials, and proteins, etc., and has been utilized in the fields such as chemical analysis, biomedicine, and environmental monitoring, etc. In the testing process, a sample with microparticles in microfluidic channels needs to be steadily positioned on the center to increase the accuracy of the detection. In general, the positioning manner includes hydrodynamic positioning and acoustic positioning, etc.
However, the conventional chips for biological detection rarely have an integrated function capable of providing image analysis and biological detection simultaneously. Therefore, the present invention provides an integrated chip with cellular molecule imaging and biological detection by utilizing the design of functional microfluidic channels. The chip includes a cell liquid chamber for air releasing and electrodes for electrochemistry detection section. The chamber can provide the storage of a sampled fluid biopsy and the usage of image capturing. The electrode portions in the electrochemistry detection section can sense the bio-electrochemical signals, so the multi-functional microfluidic channels of the chip can be utilized to provide image detection and biochemistry related detection simultaneously.
In one aspect, the present invention relates to an integrated chip for providing cell image and biochemical detection including a sequentially stacked and sealed laminate set. The laminate set includes an upper laminate, a middle laminate and a lower laminate. The first laminate is formed of a first plate, which is having one or more holes penetrating the upper laminate, the holes used for sample injection, and sample or air discharging, respectively. The middle laminate is formed of a second plate, which is including at least two hollow structures that define an imaging chamber and a biochemical detection area, respectively. The lower laminate is formed of a third plate, which is including at least one set of a filtering element and electrode sensing element that is disposed in the biochemical detection. The filtering element is for blocking suspended particles, and the electrode sensing element has an electrode section and electrode terminals that can provide connection to instruments or equipment to perform the measurements and analysis of electrochemistry and impedance.
The integrated chip of the present invention can detect the morphology of a cell and the microparticles contained therein (a specific genetic material, protein, etc.) simultaneously. The detection manners generally include the method such as electrical impedance detection, fluorescence detection, light scattering, microscopic imaging, etc.
In the preferred embodiment of the present invention, the plates of the laminate set can be made of the materials selected from light penetrable (preferably transparent) glass, plastic, acrylic, etc., and the thickness of each plate is between 50-300 micrometers.
In the preferred embodiment of the present invention, the imaging chamber can be connected to an image monitoring device that includes a microscopic image receiver and an image analysis device.
In the preferred embodiment of the present invention, the electrode sensing element includes at least a pair of microelectrodes on which electrical signals with different amplitudes and frequencies are applied (e.q., cyclic voltammetry (CV) method, the chronoamperometry method, etc.) to perform the measurements of electrochemistry.
In the preferred embodiment of the present invention, a molecule for capturing, e.q., biomolecules such as an antibody, antigen, nucleic acid, protein, etc., is modified in the electrode section to allow a target molecule present in a sample to be bound with the molecule for capturing. The electrochemical measurements for the target molecule captured on the chip can be performed using the electrochemical characteristics of the target molecule. Alternatively, a corresponding molecule carrying a detectable material, e.q., biomolecules such as an antibody, antigen, nucleic acid, protein, etc. is further introduced and bound again to perform the electrochemical measurements and analysis of the corresponding molecule via the electrode terminals.
In another aspect, the present invention relates to an image monitoring device, which comprises the integrated microfluidic chip for cell imaging and biochemical detection mentioned above, a microscopic image receiver, and an image analysis device. The imaging chamber is further connected to the image monitoring device. A microscopic image receiver is used as part of the system to receive and process images.
The invention as well as a preferred mode of use, further objectives and advantages thereof will be best understood by reference to the following detailed description of illustrative embodiments when read in conjunction with the accompanying drawings, wherein:
These and other aspects of the embodiments herein will be better appreciated and understood when considered in conjunction with the following description and the accompanying drawings.
The embodiments below are used to illustrate the present invention and are not considered as a limitation to the scope of the present invention. Unless specifically designated, the techniques used in the embodiments are ordinary skills known to the skilled in the art, and all materials are commercially available.
Referring to
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As for the shape, size, material properties, and layout of the electrodes, the document does not provide specific details. However, based on the available content, it can be inferred that the electrode design should be capable of performing electrochemical measurements, such as cyclic voltammetry (CV) and chronoamperometry. This likely implies that the electrodes have an appropriate surface area and conductivity to ensure effective electrochemical reactions and signal detection. The material properties may include the use of highly conductive materials, such as gold, platinum, or carbon-based materials. In terms of layout, the electrodes might be designed to be compatible with the filtering structure 108 and microarrays 109, allowing for immediate analysis of samples after filtration. The specific size and shape would depend on the desired electrochemical performance and integration with other microfluidic structures.
Therefore, after filtration, the sample can undergo electrochemical analysis immediately, significantly reducing the risk of inaccuracies in the analysis results caused by impurities affecting the sample within the flow channel. By minimizing the distance and time between filtration and detection, the system can effectively reduce contamination and external interference, thereby enhancing the accuracy and reliability of the measurements.
The shape and size of the electrode section 1071 can affect the power density and energy density. For example, porous electrodes can increase the surface area of the electrode section 1071, thereby enhancing the charge and discharge rates. The choice of electrode materials is crucial for the performance. Materials with good conductivity can reduce internal resistance losses and improve energy conversion efficiency. Additionally, the stability and durability of the materials also impact the lifespan and safety of the electrode sensing element 107. The layout design of the electrode section 1071 affects the internal electron and ion transport within the electrode sensing element 107. An optimized layout can reduce transport distances, improving the reaction rate and efficiency.
As shown in
The microbeads 1092 are typically small, spherical particles ranging in size from a few micrometers to several hundred micrometers. Their spherical shape allows them to flow well and distribute evenly in fluids. Structurally, the microbeads 1092 are usually independent particles, easily modified on their surfaces to achieve specific functions. They can be solid or hollow and made from a variety of materials, such as polymers, glass, or magnetic substances, but is not limited thereto.
In the integrated chip of the present invention, the imaging chamber 1051 and biochemical detection area 1061 defined by the hollow structures 105 and 106, respectively, can be intercommunicated with each other or be independent. In the design of being intercommunicated with each other, one or more connecting channels 110 are disposed between the imaging chamber 1051 and the biochemical detection area 1061. A filtering element, which is the same as or similar with the aforementioned filtering element, can be disposed in the connecting channels 110 and has a filtering area 112 constructed by one or more microarrays in the form of a pillar, slot, or fence. The image of cells and micromolecules moving into the imaging chamber 1051 can be captured by a variety of image capturing devices or microscope imaging systems. The captured image can be further recorded and analyzed after being transmitted to an image analyzing equipment by a receiver.
Electrode sensing element 107, used to perform biochemical and electrical operations or analysis, includes dielectrophoresis control, impedance analysis, and electrochemical measurements, etc. Modifications can be done in the electrode sensing element 107 to assist the detection of biochemical specificity. For example, a molecule for capturing (e.q., the biomolecules such as an antibody, antigen, nucleic acid, protein, etc.) can be modified on the electrode sensing element 107. A target molecule will be bound with the capture molecule when the target to be detected passes through, then the electrochemical measurements for the target molecule can be performed using its electrochemical characteristics. Alternatively, a corresponding detected molecule (e.q., a biomolecule such as an antibody, antigen, nucleic acid, protein, etc., which carries a detectable material) is further introduced and bound with the target molecule captured on the electrode sensing element 107 to perform the electrochemical measurements and analysis for the detected molecule in the electrode section 1071 in accordance with the electrochemical characteristics of the detected molecule.
A sample to be tested, which may be a liquid sample or cell culture retrieved from a patient, is injected into the hole 104 defined by the upper laminate 101 of the chip 100. The liquid sample flows into the imaging chamber 1051 and biochemical detection area 1061 that are defined by the hollow structures 105 and 106 of the middle laminate 102, respectively, via microfluidic channels.
The image of cells in the fluid sample that flows into the imaging chamber 1051 defined by the hollow structure 105 can be captured by a variety of image capturing devices or microscope imaging systems. The image of cells can be analyzed by a microscopic image analysis and interpretation system to determine morphology and pathological conditions of the specific cell.
When the fluid sample flowing into the biochemical detection area 1061 passes through the microarray area of the filtering element 108 disposed on the lower laminate 103, the suspended particles (including macromolecules, cells, or debris thereof, etc.) in the fluid sample can be blocked outside the filtering microarrays 109 because of the filtering microarrays 109 in the form of a pillar, slot, fence, or sieve. Accordingly, only the micromolecules in the sample are allowed to pass through the filtering element 108 and move into the electrode sensing element 107 for electrochemical measurements.
One embodiment of the present invention is directed to an image monitoring device, which comprises the integrated microfluidic chip for cell imaging and biochemical detection mentioned above, a microscopic image receiver 20, and an image analysis device 21. The imaging chamber 1051 is further connected to the image monitoring device. A microscopic image receiver 20 is used as part of the system to receive and process images.
The image analysis device 21 should be positioned to receive image signals from the microscopic image receiver 20. This means it should be directly connected to the microscopic image receiver 20 or linked via data transmission lines (such as USB, Ethernet, or wireless connections) to receive and process these images. In practical implementations, the image analysis device 21 may be a dedicated computer system equipped with a powerful processor and specialized analysis software for detailed examination of the received images.
The primary function of the microscopic image receiver 20 is to receive microscopic images from the imaging chamber 1051 and transmit these images to image analysis equipment for recording and analysis. During the image acquisition process, the microscopic image receiver 20 connects to various image capture devices or microscope imaging systems. When a liquid sample enters the imaging chamber 1051, images of the cells or particles within the sample are captured by these devices.
The microscopic image receiver 20 can be a photosensitive element or a camera, but is not limited thereto. The microscopic image receiver 20 is used to receive optical signals and convert them into digital signals for further processing and analysis. In an implementation example, a microscope imaging system is used for image acquisition, and the microscopic image receiver 20 is compatible with the image analysis device 21, enabling it to receive and process magnified images.
The image analysis device 21 included in the image monitoring device is designed to handle a variety of biochemical assays. This device can process data from different biochemical reactions, including enzyme reactions and molecular marker assays. The image analysis device 21 is equipped with advanced algorithms and software that allow it to analyze these results comprehensively. It integrates data from multiple sources, providing a unified analysis of biochemical reactions. This capability enables users to obtain a holistic view of the biochemical processes occurring within the imaging chamber 1051, improving the accuracy and relevance of the assay results.
The microscopic image receiver 20 in the image monitoring device is designed to work in conjunction with micro sensors embedded in the integrated microfluidic chip. This synchronization allows for real-time monitoring of biochemical reactions occurring on the chip. By coordinating with the micro sensors, the image receiver captures images that reflect the current state of biochemical processes, providing immediate feedback on reaction dynamics. This real-time capability is crucial for observing transient or rapid biochemical events, ensuring timely and accurate data collection for subsequent analysis.
In one embodiment, the image monitoring device is equipped with an adaptive control system that monitors cell images and automatically adjusts the parameters of the integrated microfluidic chip. As the cell images are analyzed, the device can detect changes or variations in the cellular environment or biochemical processes. Based on this real-time analysis, the device adjusts parameters such as fluid flow rates, reagent concentrations, or imaging settings to optimize the conditions for cell imaging and biochemical detection. This dynamic adjustment capability enhances the accuracy and sensitivity of the assays by ensuring that the chip operates under optimal conditions throughout the experiment.
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The preferred embodiments above are merely exemplary, the present invention may include various embodiments described in this description and other embodiments. Further, the above-mentioned embodiments are merely illustrations of the present invention and are not limiting. Other equivalent variations and modifications done without departing the spirit disclosed by the present invention shall be included in the claims described below.
While the present invention has been described in terms of what are presently considered to be the most practical and preferred embodiments, it is to be understood that the present invention need not be restricted to the disclosed embodiment. On the contrary, it is intended to cover various modifications and similar arrangements included within the spirit and scope of the appended claims which are to be accorded with the broadest interpretation so as to encompass all such modifications and similar structures. Therefore, the above description and illustration should not be taken as limiting the scope of the present invention which is defined by the appended claims.
| Number | Date | Country | |
|---|---|---|---|
| Parent | 17543728 | Dec 2021 | US |
| Child | 18893264 | US |
