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Sonication aided exosomes drug loading

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Sonication Aided Exosomes Drug Loading

Exosomes are natural, intrinsic, cell-derived inter-cellular communication phospholipid membrane nanovesicles in the size range of 40-100 nm. Besides carrying several cell-derived growth factor, they can serve as a great tool for intracellular drug delivery.

These biologically natural nanocarriers possess many advantages such as:

1- They are known to bypass biological barriers, such as the blood-brain barrier.

2- Exosomes have the property of homing, making them helpful in tissue targeting.

3- High biocompatibility.

4- Cargo protection from degradation.

Due to these promising properties exosomes can be used as drug delivery carrier.

Category: Stem Cells Tags: articular cartilage, burns, cytotoxicity, diabetes, drug carriers, drug delivery, exosomes, genetics, mesenchymal stem cells, metastasis, myocardial infarction, nanotechnology, neurodegenerative diseases, osteoarthiritis, purification, quantification, regenerative medicine, scaffolds, skin wounds, tissue engineering, ulcers, ultracentrifugation., vaccination
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Description

Sonication Aided Exosomes Drug Loading

Exosomes are natural, intrinsic, cell-derived inter-cellular communication phospholipid membrane nanovesicles in the size range of 40-100 nm. Besides carrying several cell-derived growth factor, they can serve as a great tool for intracellular drug delivery.

These biologically natural nanocarriers possess many advantages such as:

1- They are known to bypass biological barriers, such as the blood-brain barrier.

2- Exosomes have the property of homing, making them helpful in tissue targeting.

3- High biocompatibility.

4- Cargo protection from degradation.

Due to these promising properties exosomes can be used as drug delivery carrier.

Procedure:

1-    measuring exosome concentration using BCA assay kit or Bradford assay.

2-    Exosomes are diluted in PBS to a concentration 0.15 mg/mL total protein.

3-    Determination of the drug solubility to determine the used solvent (PBS or DMSO).

4-    Post loading strategy; the drug solution in PBS (0.5 mg/mL) was added to 250 µl of exosomes to the final concentration 0.1 mg/mL total protein.

Illustration:

125 ul (drug) added to 250 ul EXO

MV=MV

150×250=100V2

V2=375 µl

Therefore, 125 µl Drug+250 µl EXO =375 total volume

5-    Drug-EXO mixture is sonicated using probe sonicator (750 v, 20% power, 6 cycles by 4 sec pulse /2 sec pause (total time 24 sec), cooled down on ice for 2 min, and then sonicated again.

Note: 1-it is preferred to put the EXO-DRUG mixture in falcon tube during sonication to avoid loss of volume during sonication.

6-    Incubation in 37 °C for 1 hr without shaking (The membrane integrity of the exosomes has been found to be restored within an hour when the exosomes are incubated at 37 °C).

7-    Put 300 ul of the EXO-DRUG mixture in Nanosep. (or in dialysis sac)

8-    Centrifugation (cooling) 7500 rpm for 15 min for 2 runs (twice).

9-    The amount of Drug loaded into exosomes was measured by a high-performance liquid chromatography (HPLC) or any suitable device (GC-mass – ICP) method according of the drug.

10- To ensure the exosomes integrity and structure we can confirm using TEM.

Refrences:

Haney, M. J., Klyachko, N. L., Zhao, Y., Gupta, R., Plotnikova, E. G., He, Z., … & Batrakova, E. V. (2015). Exosomes as drug delivery vehicles for Parkinson’s disease therapy. Journal of controlled release, 207, 18-30.

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1- Cytotoxicity assays
2- Cell migration / Wound healing assay
3- Western Blotting
4- Quantitative PCR services (qPCR).
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6- PCR primer design and validation

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