Protein Electrodialiysis (PED) Device for Enrichment of the Extracellular Proteins Deposited by Microorganisms in Liquid Culture
20190112332 ยท 2019-04-18
Inventors
Cpc classification
B01D2313/06
PERFORMING OPERATIONS; TRANSPORTING
C07K1/34
CHEMISTRY; METALLURGY
C12M47/10
CHEMISTRY; METALLURGY
International classification
C07K1/36
CHEMISTRY; METALLURGY
C07K1/34
CHEMISTRY; METALLURGY
Abstract
An efficient tool with low cost to rapidly isolate and concentrate the secreted proteins of microorganisms in high quality. By this device, the secreted proteins are concentrated by passing through a dialysis membrane at electrophoretic conditions.
Claims
1- A Protein Electrodialysis (PED) device comprising: A holder; a main container; a harvesting container; a dialysis membrane and power supply; wherein said holder is a metallic backing, holding said main container and said harvesting container in a desired position with respect to each other; wherein said main container comprises an open end and a closed end, wherein said closed end is cut open and covered with a sheet of plastic of said dialysis membrane using plastic glue; and wherein said harvesting container is a plastic container placed facing and under said dialysis membrane.
2- The device of claim 1, wherein said membrane has a molecular weight cut off of 12 KDa.
3- The device of claim 2, wherein said main container comprises a predetermined quantity of an enriched protein (centrifuged liquid culture medium); and said harvest container comprises a buffer.
4- The device of claim 3, wherein said power supply comprises an anode and cathode end; wherein one end (said anode) is located inside said main container touching said culture medium and the other end (said cathode) is located inside said harvest container being in contact with said buffer; wherein when said power supply is turned on, a second quantity of molecules of said enriched protein move from said main container into said harvesting container.
5- The device of claim 4, wherein said predetermined quantity of said enriched protein is at most 50 ml and said second quantity is at least 3 ml.
6- The device of claim 5, wherein said culture medium comprises but not limited to carboxy methyl cellulose (CMC) medium containing 0.05 g FeSO4 7H2O, 0.25 g MnSO4 H2O, 0.25 g CoC12, 0.25 g ZnSO4, 0.25 g (NH4)2SO4, 2 g KH2PO4, 0.25 g MgSO4 7 H2O, 0.4 g CaCl2, 0.3 g urea, 0.2 ml Tween 80 and 10 g Carboxy Methyl Cellulose per liter.
7- The device of claim 6, wherein said buffer comprises Tris-Hcl with pH=7.
Description
BRIEF DESCRIPTION OF DRAWINGS
[0017]
[0018]
[0019]
LIST OF ALL ITEMS
[0020] The following is the list of all the components used in this invention as well as a brief description of each piece: [0021] 1 Column/main container: A 50 ml plastic column tube (Falcon, USA) selected as column [0022] 2 Centrifuged Liquid Culture Medium: The liquid culture medium inside the column has already been centrifuged at 2000 rpm for 5 min to remove any fungi mycelium/bacteria. [0023] 3 Dialysis Membrane: The bottom of the main container/column (1) was cut and covered with a sheet of plastic dialysis membrane (3) with molecular weight cut-off 12 KDa. The membrane was fixed using plastic glue. [0024] 4 Harvesting container: A plastic container was placed under the dialysis membrane (3). [0025] 5 The Buffer of Harvesting Container: The Harvesting Container (4) was filled with a buffer (e.g.Tris-Hcl pH=7). [0026] 6 Holder: A metallic backing holds the main container/column (1) and the harvesting container (4). [0027] 7 Anode: The negative electrode made of platinum was placed above the column [0028] 8 Cathode: The positive electrode made of platinum was placed in the harvesting container (4). [0029] 9 Power supply: The power supply was used to provide the electric energy needed for moving proteins across the column (1) and through the dialysis membrane (3).
DETAILED DESCRIPTION OF SPECIFICATION
[0030] The subject of electrophoresis deals with the controlled motion of charged particles in electric fields. Since proteins are charged molecules, they migrate under the influence of electric fields. The electrophoresis mobility of a protein depends on its charge, size and shape.
[0031] For enrichment of the proteins; the liquid culture medium was centrifuged at 2000 rpm at 5 min to remove fungi mycelium/bacteria. Then as much as 50 ml of the centrifuged liquid culture medium (2) was poured into the main container (1), afterwards the electric charge (15 mA) was set in the device using the power supply (9). In this device, the electric field between the liquid culture medium (2) and the buffer inside the harvesting container (5) leads to the movement of protein molecules from the negative electrode (7) at top of the column to the positive electrode (8) in the buffer of the harvesting container (5). At the end of the procedure, as much as 3 ml of protein molecules would be concentrated in the buffer of the harvesting container (5).
Reliability
[0032] To check the performance of the device and the results obtained from, we designed an experiment detailed as follows:
[0033] Fungal isolate: Isolation of Trichoderma harzianum was grown on PDA medium and stored at 4? C.
[0034] Culture medium: carboxy methyl cellulose (CMC) medium containing 0.05 g FeSO4 7H2O, 0.25 g MnSO4 H2O, 0.25 g CoC12, 0.25 g ZnSO4, 0.25 g (NH4)2SO4, 2 g KH2PO4, 0.25 g MgSO4 7 H2O, 0.4 g CaCl2, 0.3 g urea, 0.2 ml Tween 80 and 10 g Carboxy Methyl Cellulose per liter were prepared for cellulose degradation experiments. Fifty milliliter of broth was distributed in 250 ml Erlenmeyer and then media was autoclaved at 120? C. for 20 min.
[0035] Inoculation and sampling: Flask was inoculated with 1 ml spore suspension in three replicates for each species. The flasks were treated at 25? C. for 31 days and then medium culture centrifuged at 2000 rpm for 5 min.
[0036] Protein electrodialysis (PED): Fifty ml of the centrifuged culture medium was poured into the column (main container) and the anode electrode was fixed in the liquid culture medium (2) at top of the column (1); while the cathode electrode was put into the buffer of the harvesting container (5). Then the power supply was set at 15 miliA.
[0037] Quantification of Protein and the reduced sugar: To check the performance of the device, the amount of cellulose enzyme and the related substrate (reduced sugar assay) were measured at top of the column, bottom of the column and inside the harvesting container. To do that, sampling (50 ?l) was done at each 15 min time point for 120 min. Released fungal extracellular proteins and produced sugars concentrations were determined using Bradford method and Arsenate-Molybdate reagent assay, respectively (Bradford, 1976; Kossem and Nannipieri, 1995).
[0038] Results: Based on our results the protein content gradually decreased at top of the column; while increased at down of the column throughout 90 min after beginning the Protein electrodialysis (PED). On the other hand, the amount of the protein increased in the harvesting container at 45 min after the beginning of the experiment (
[0039] The PED device of this invention is a low cost and user friendly laboratory instrument that concentrates secreted proteins/enzymes obtained from microorganisms such as filamentous fungi and bacteria. It can be used to concentrate proteins/enzymes secreted by microorganisms which have been grown in liquid culture medium. Also proteins inside any liquid culture media can be concentrated by PED after centrifugation at 2000 rpm for 5 min. Up to 50 ml of liquid culture medium can be used to concentrate the secreted proteins/enzymes using PED. It is suggested to use PED at cold room temperature, where it can be used in a variety of small and large biotechnology laboratories.