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US20040178071A1 - Microfluidic system and methods of use - Google Patents

Microfluidic system and methods of use
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Publication number
US20040178071A1
US20040178071A1US10/637,689US63768903AUS2004178071A1US 20040178071 A1US20040178071 A1US 20040178071A1US 63768903 AUS63768903 AUS 63768903AUS 2004178071 A1US2004178071 A1US 2004178071A1
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United States
Prior art keywords
flow path
cells
detection zone
inlet flow
cell
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Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Abandoned
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US10/637,689
Inventor
Daniel Harrison
Paul Li
Roderick Szarka
Richard Smith
Per Anderson
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University of Alberta
Alberta Innovates
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University of Alberta
Alberta Innovates
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Application filed by University of Alberta, Alberta InnovatesfiledCriticalUniversity of Alberta
Priority to US10/637,689priorityCriticalpatent/US20040178071A1/en
Publication of US20040178071A1publicationCriticalpatent/US20040178071A1/en
Abandonedlegal-statusCriticalCurrent

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Abstract

This invention relates to a novel microfluidic device and methods of using this device to conduct in vitro studies on the reaction and effects of various compounds on cells. More particularly, it relates to a method for using stop flow in a microfluidic system to study the effect of compounds on individual cells.

Description

Claims (34)

We claim:
1. A microfluidic device comprising:
a main flow path comprising a detection zone and an outlet; and
at least two inlet flow paths wherein the inlet flow paths intersect and merge into the main flow path at or upstream of the detection zone at an upstream angle of less than 90°.
2. The microfluidic device ofclaim 1 further comprising two inlet flow paths.
3. The microfluidic device ofclaim 1 further comprising three inlet flow paths.
4. The microfluidic device ofclaim 3 wherein the main flow path has at least one detection zone at or downstream of each intersection of each inlet flow path with the main flow path.
5. The microfluidic device ofclaim 1 wherein the main flow path is from about 0.1 μm deep by 0.1 μm wide to about 1 mm deep by 2 mm wide.
6. The microfluidic device ofclaim 1 wherein the first inlet flow path is from about 0.1 μm deep by 0.1 μm wide to about 1 mm deep by 2 mm wide.
7. The microfluidic device ofclaim 1 further comprising means for applying a flow inducing force.
8. The microfluidic device ofclaim 6 wherein the flow inducing force is electricity.
9. The microfluidic device ofclaim 6 wherein the flow inducing force is negative or positive fluid pressure.
10. The microfluidic device ofclaim 9 wherein positive or negative pressure is applied to the outlet.
11. The microfluidic device ofclaim 1 wherein the device further comprises cells in at least one of the inlet flow paths and the main flow path.
12. The microfluidic device ofclaim 1 wherein the device further comprises leukocytes, a calcium dye and a candidate compound in the main flow path.
13. An observation device comprising a plurality of microfluidic devices ofclaim 1 sharing a common detection zone.
14. The observation device ofclaim 13, wherein the main flow paths of the microfluidic devices are substantially parallel at the common detection zone.
15. An observation device comprising a plurality of microfluidic devices ofclaim 1 wherein the main flow paths of the microfluidic devices are substantially parallel at their detection zones.
16. A method of observing the effect of a candidate compound on cells in a microfluidic device comprising:
(a) providing a microfluidic device comprising a main flow path comprising a detection zone, and an outlet and at least two inlet flow paths intersecting and merging with the main flow path at or upstream of the detection zone;
(b) applying at least one cell to a first inlet flow path and the candidate compound to a second inlet flow path;
(c) inducing flow of the cells and the candidate compound toward the outlet;
(d) allowing the cells to mix with the candidate compound at the intersection of the second inlet flow path and the main flow path; and
(f) observing the effect of the candidate compound on the cells in the detection zone.
17. The method ofclaim 16 wherein the microfluidic device has three inlet flow paths and a second candidate compound is added to the third inlet flow path.
18. The method ofclaim 16 further comprising stopping the flow of the cells while the cells are in the detection zone.
19. The method ofclaim 17 further comprising observing the cells in each of a number of detection zones wherein the main flow path comprises a plurality of detection zones, wherein each detection zone is at or downstream of each intersection of each inlet flow path with the main flow path.
20. The method ofclaim 16 wherein the candidate compound being studied is a cell activator and the cell is a lymphocyte.
21. The method ofclaim 17 wherein cells are added to a first inlet flow path, cell activator is added to a second inlet flow path, and a candidate compound is added to a third inlet flow path.
22. The method ofclaim 21 wherein the candidate compound being studied is an inhibitor, and the cells are lymphocytes.
23. The method ofclaim 16 wherein the flow paths are coated with a substance selected from the group consisting of proteins, glycoproteins, phospholipids, hydrophilic polymers and hydrophobic polymers.
24. The method ofclaim 23 wherein the flow path is coated with protein.
25. The method ofclaim 23 wherein the flow is induced by an electric force.
26. The method ofclaim 24 wherein the flow is induced by positive or negative fluid pressure.
27. A method for studying calcium influx in a lymphocyte comprising:
(a) providing a microfluidic device comprising a main flow path having a detection zone, at least two inlet flow paths sequentially intersecting with the main flow path upstream of the detection zone and an outlet downstream from the detection zone;
(b) applying lymphocytes to a first inlet flow path and an activator to a second inlet flow path;
(c) inducing flow of the lymphocytes and the activator toward the outlet;
(d) allowing the lymphocytes to mix with the activator at the intersection of the second inlet flow path and the main flow path; and
(e) observing the effect of the activator on the lymphocytes in the detection zone.
28. The method ofclaim 27 wherein the microfluidic device comprises three inlet flow paths further comprising adding a candidate compound to a third inlet flow path; and observing the effect of the candidate compound on the lymphocytes in the detection zone.
29. A method for studying leukocyte rolling comprising:
(a) providing a microfluidic device comprising a main flow path comprising a detection zone and an outlet and at least two inlet flow paths sequentially intersecting and merging with the main flow path at or upstream of the detection zone and wherein the walls of the main flow path in the detection zone have attached thereto cell adhesion molecules;
(b) applying at least one leukocyte to a first inlet flow path;
(c) applying a candidate compound to a second inlet flow path;
(d) inducing flow of the cells and the compound into the main flow path;
(d) allowing the leukocytes, candidate compound and cell adhesion molecules to interact; and
(e) observing the leukocyte rolling in the detection zone.
30. The method ofclaim 29 wherein the device comprises three inlet flow paths, further comprising adding an inhibitor to said third inlet flow path; mixing the inhibitor, leukocytes, candidate compound and cell adhesion molecules and observing the leukocyte rolling in the detection zone.
31. The method ofclaim 30 further comprising stopping the flow of the cells, candidate compound and inhibitor during the mixing step.
32. The device ofclaim 1 further comprising variations in the cross-section of the main flow path.
33. The device ofclaim 32 wherein the variations create a cell trapping zone.
34. The device ofclaim 33 wherein said variations are weirs.
US10/637,6891997-05-162003-08-11Microfluidic system and methods of useAbandonedUS20040178071A1 (en)

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US10/637,689US20040178071A1 (en)1997-05-162003-08-11Microfluidic system and methods of use

Applications Claiming Priority (2)

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US08/858,087US6632619B1 (en)1997-05-161997-05-16Microfluidic system and methods of use
US10/637,689US20040178071A1 (en)1997-05-162003-08-11Microfluidic system and methods of use

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