Patent Grant
8632243
Microfluidics refers to the design and use of fluid systems in which at least one dimension is smaller than 1 mm. Fluid flow in microfluids systems can be characterized as either laminar or turbulent. Turbulent flow is chaotic on a small scale, such as tap water turned on at full blast. Laminar flow consists of fluid flowing in layers in which the velocity at a given time and place is invariant under steady-state conditions. Due to the small size of microfluidic systems, laminar flow predominates. A key aspect that contributes to both the advantages and disadvantages of laminar flow is the absence of convective transport between adjacent layers of fluid. This lack of convection poses clear problems in terms of successful on-chip mixing, after leading to non-diffuse or poorly mixed solutions.
It is an object of the present invention to overcome the disadvantages and problems in the prior art.
The present invention relates to a method for microfluidic mixing in a “lab-on-a-chip” environment. The methodology focuses on continuous acceleration and deceleration about a mean angular speed with a rotating platform serving as the mixing platform. The methodology results in good mixing between different species. The rotating platform can be read by an optical analyzer that may be stationery or portable.
These and other features, aspects, and advantages of the apparatus and methods of the present invention will become better understood from the following description, appended claims, and accompanying drawings where:
The following description of certain exemplary embodiment(s) is merely exemplary in nature and is in no way intended to limit the invention, its application, or uses. Throughout this description, the terms “diffusion”, “diffused”, or “diffuse” shall refer to the state or process of the spontaneous movement of particles and/or species in a solution toward a uniform concentration with another species. The term “species” can refer to a homogeneous fluid, fluid with suspended solids, liquid with dissolved solids, liquid with both dissolved solids and suspended solids, two mixable liquid mixture with one dissolved in the other, for example water dissolved in glycerine/glycerol or water in alcohol. The term “fluids” shall refer to a material or combination of materials that is liquid at room temperature and one atmosphere. The term “lab-on-a-chip” refers to capabilities for fast chemical/biological analysis of a specimen using microfluidic volumes of species. The phrase “microfluidic volume” refers to volumes equal to or less than 1000 μL.
Now, to
In a first step, two or more fluids are added to the cavity in a rotating platform 101. As known in the art, microfluidic “lab-on-a-chip” environments allow the usage of microfluidic volumes of species during analysis. Species volumes can be 1-1000 μL, alternatively 1-100 μL, individually or collectively. Species can be added by methods well-known in the art, such as pipetting.
The rotating platform useful in the present method can be made of a silicone or glass substrate. The rotating platform can be from around 6 to about 13 centimeters in diameter, and from 0.1 to 1 mm in thickness. The rotating platform possesses a cavity capable of accepting the species.
In the next step, the rotating platform is positioned and placed in an analyzer 103. The analyzer can be portable or a lab-bench design. Positioning the rotating platform in the analyzer can include physically placing the rotating platform in the reader of the analyzer.
Upon being in the analyzer, a determination is made as to whether the species are at least sufficiently diffused with one another 105. Sufficient diffusion refers to the fluids not being 100% diffused into one another, but above 50% diffusion volume-to-volume. If not yet diffused, the rotating platform is then accelerated 107 and decelerated 109 to a minimum speed in a methodology allowing good mixture of the species. Maximum speed and minimum speed of the rotating platform can occur over a mean angular speed. In one embodiment, a mean angular speed of around 10 rev/min is set, with a maximum speed of 15 rev/min and minimum speed of 5 rev/min. Acceleration and deceleration can occur, for example, over a 10 minute cycle. During acceleration 107 and deceleration 109, a determination is made as to whether the species in the rotating platform's cavity have become sufficiently diffused. In the event the species become sufficiently diffused, the resultant mixture is then scanned for a desired analyte 111. If the species are not sufficiently diffused, the rotating platform is accelerated and decelerated again.
In another embodiment, intense mixing and violent agitation can be effected by circulatory flow that relies upon high rotation speed, i.e., over 1000 rev/min, and a large time rate of change in rotation speed.
Having described embodiments of the present system with reference to the accompanying drawings, it is to be understood that the present system is not limited to the precise embodiments, and that various changes and modifications may be effected therein by one having ordinary skill in the art without departing from the scope or spirit as defined in the appended claims.
In interpreting the appended claims, it should be understood that:
a) the word “comprising” does not exclude the presence of other elements or acts than those listed in the given claim;
b) the word “a” or “an” preceding an element does not exclude the presence of a plurality of such elements;
c) any reference signs in the claims do not limit their scope;
d) any of the disclosed devices or portions thereof may be combined together or separated into further portions unless specifically stated otherwise; and
e) no specific sequence of acts or steps is intended to be required unless specifically indicated.
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