A computer readable XML file entitled “GWP20230503728_seqlist”, that was created on Aug. 17, 2023, with a file size of about 3,894 bytes, contains the sequence listing for this application, has been filed with this application, and is hereby incorporated by reference in its entirety.
The present disclosure relates to the field of biomedicine, in particular to a drug delivery system for delivering a drug to cells, and a preparation method and a use method thereof.
Small-molecule transdermal drug delivery is to deliver small-molecule drugs through a skin barrier into the body to produce pharmaceutical effects. However, many drugs need to enter cells to express related proteins to produce corresponding pharmaceutical effects. These drugs mainly include but not limited to nucleic acid drugs. Currently, methods for delivering such drugs into cells include lipofection, electroporation, gene gun, and viral transfection. Liposomes have been extensively studied as delivery carriers in vivo and in vitro. Nucleic acid drugs encapsulated in synthetic liposomes can also enter human cells through fusion. The electroporation refers to a technique in which small holes or openings are temporarily formed on the cell membrane under the action of an electric field, and nucleic acid drugs enter cells through such small holes or openings. The gene gun is to temporarily form some pores in the cell membrane using high-pressure gas as an accelerating force, and pushes nucleic acid drugs coated on a surface of gold particles into the host cells. The viral transfection is to construct a virus vector, infect a host cell with the virus vector, and integrate a gene into the host cell.
In view of this, the technical problem to be solved by the present disclosure is to overcome the defects of low transfection efficiency, relatively complicated operation during preparation, and high application cost in the prior art when delivering nucleic acid drugs to cells.
On one hand, an example of the present disclosure provides a drug delivery system, including a drug delivery carrier, where a nucleic acid drug and a photothermal nanoparticle are encapsulated in the drug delivery carrier.
Optionally, the nucleic acid drug is selected from the group consisting of a DNA drug or an RNA drug.
Optionally, the system further includes an infrared laser emitter, where the infrared laser emitter has an emission wavelength of 760 nm to 1 mm.
Optionally, the infrared laser emitter is a near infrared laser emitter; and the infrared laser emitter has an emission wavelength of 760 nm to 2,526 nm and an illumination density of 3 W/cm2 to 4 W/cm2.
Optionally, the infrared laser emitter has an emission wavelength of 808 nm and an illumination density of 4 W/cm2.
Optionally, the photothermal nanoparticle is selected from the group consisting of a compound of a metal and a non-metal, a metal nanoparticle, and a non-metal nanoparticle.
Optionally, the compound of the metal and the non-metal is Mxene; the metal nanoparticle is selected from the group consisting of a gold nanoparticle and a platinum nanoparticle; and the non-metal nanoparticle is selected from the group consisting of polydopamine (PDA) and graphene oxide (GO).
Optionally, the drug delivery carrier is a microneedle patch.
Optionally, 100 ng to 600 ng of the nucleic acid drug is encapsulated based on a microneedle patch of a 10*10 array.
Optionally, the microneedle patch includes raw materials of polyvinylpyrrolidone (PVP) and hyaluronic acid (HA); the PVP has a molecular weight of 8 kDa to 11 kDa, and the HA has a molecular weight of 3.9 WDa; and the PVP and the HA are at a mass fraction ratio of (10-30):3.
Optionally, the PVP and the HA are at a mass fraction ratio of 20:3.
Optionally, a microneedle patch backing is prepared from PVP with a molecular weight of 32 WDa to 38 WDa.
On the other hand, an example of the present disclosure provides a preparation method of a drug delivery system, where the drug delivery system includes a microneedle patch encapsulating a nucleic acid drug and a photothermal nanoparticle; and
On the other hand, an example of the present disclosure further provides a use method of a drug delivery system, where the drug delivery system includes a microneedle patch encapsulating a nucleic acid drug and a photothermal nanoparticle; and the use method includes the following steps:
The technical solutions of the present disclosure have the following advantages:
To describe the technical solutions in the specific implementations of the present disclosure or the prior art more clearly, the accompanying drawings required for describing the specific implementations or the prior art are briefly described below. Apparently, the accompanying drawings in the following description show merely some implementations of the present disclosure, and a person of ordinary skill in the art may still derive other accompanying drawings from these accompanying drawings without creative efforts.
The following examples serve to provide further appreciation of the present disclosure, but are not limited to the preferred examples and do not limit the spirit and scope of the disclosure; any product that is the same as or similar to the disclosure made in light of the disclosure or by combination of the present disclosure with other features of the prior art shall fall within the scope of the disclosure.
If specific experimental procedure or conditions are not indicated in the present disclosure, operations or conditions of conventional experimental procedures known in the art shall be used. If manufacturers of reagents and apparatus used are not indicated, conventional reagent products may be commercially available.
An example of the present disclosure provides a drug delivery system for delivering a drug to cells, including a drug delivery carrier, where a nucleic acid drug and a photothermal nanoparticle are encapsulated in the drug delivery carrier.
The nucleic acid drug can be a DNA drug or an RNA drug.
In the example of the present disclosure, the drug delivery system further includes an infrared laser emitter, where the infrared laser emitter has adjustable power; and the infrared laser emitter has an emission wavelength of 760 nm to 1 mm. In one embodiment, the infrared laser emitter can be a near infrared laser emitter, with an emission wavelength of 760 nm to 2,526 nm and an illumination density of (3-4) W/cm2, further preferably an emission wavelength of 808 nm and an illumination density of 4 W/cm2.
In an example of the present disclosure, the drug delivery carrier may be a microneedle patch. As shown in
The microneedle patch backing is prepared from PVP with a molecular weight of (32-38) WDa.
An amount of the nucleic acid drug can be controlled according to the addition of drugs with different concentrations; the nucleic acid drug is a DNA drug or an RNA drug. In this example, the nucleic acid drug is loaded with a plasmid expressing a green fluorescent protein (GFP) (plasmid GPC, with a nucleic acid sequence shown in SEQ ID NO: 1).
In an example of the present disclosure, the photothermal nanoparticle is selected from the group consisting of a compound of a metal and a non-metal, a metal nanoparticle, and a non-metal nanoparticle. Optionally, the compound of the metal and the non-metal is Mxene; the metal nanoparticle is selected from the group consisting of a gold nanoparticle and a platinum nanoparticle; and the non-metal nanoparticle is selected from the group consisting of PDA and GO. The photothermal nanoparticle can be the Mxene (Shandong Xiyan New Material Technology Co., Ltd.).
In this example, a microneedle patch of a 10*10 array is prepared. The height of the microneedle patch is 670 μm, the size of the needle tip is 15 μm, the size of the bottom of the microneedle is 300*300 μm. The microneedle patch is a quadrangular pyramid, the distance between the centers of two adjacent microneedles is 500 μm, the size of the backing is 9.8*9.8 mm, and a backing thickness is 1.5 mm. The specific size and shape of the microneedle can be changed according to experimental needs. Each microneedle patch (the microneedle patch of the 10*10 array) encapsulates a nucleic acid drug (in the experiment, a plasmid that encodes GFP, namely a plasmid GPC) in an amount of 500 ng, and encapsulates nanoparticles (in this example, Mxene) in an amount of 536 ng. The specific amounts of nucleic acid drug and nanoparticles can be changed according to experimental needs. The microneedle backing material is PVP with a molecular weight of (32-38) WDa.
500 ng of the plasmid GPC is encapsulated in each 10*10 array of microneedle patch.
The example of the present disclosure further provides a preparation method of the drug delivery system. Take a preparation method of a microneedle patch encapsulating a nucleic acid drug and a photothermal nanoparticle as an example, the preparation method was described as follows.
A configuration method of a 1 g/ml PVP solution included:
A configuration method of a 150 mg/ml HA solution included:
Step I: a microneedle material was selected.
Microneedle patch materials included PVP with a molecular weight of (8-11) kDa at a concentration of 1 g/ml and HA with a molecular weight of 3.9 WDa at a concentration of 150 mg/ml. A microneedle backing working solution was PVP with a molecular weight of (32-38) WDa.
Step II: a microneedle working solution was prepared, including a needle tip (i.e.) working solution and a backing working solution.
The microneedle backing working solution was a PVP solution with a concentration of 0.5 g/ml.
The needle tip working solution was described by taking the preparation of 400 μl of the needle tip working solution as an example. A PVP solution, an HA solution, and a photothermal nanoparticle solution were at a volume ratio of (2-4):(2-4):1. Specifically,
Therefore, 66.96 μl of a 1.6 mg/ml Mxene solution and 65.2 μl of a 1335.2 ng/μl GPC solution were added to the mixed solution 1, shaken fully, and vacuumed to remove air bubbles in the working solution, to obtain a uniform needle tip working solution.
Step III: after the two working solutions were prepared, the PDMS concave mold was removed to start making the microneedle.
The needle tip working solution was pipetted into the PDMS concave mold with a pipette gun, where it was necessary to ensure that the needle tip working solution covered a pinhole array of the mold. Vacuum extraction was conducted in a vacuum pump with a pressure of −103 kPa for 3 h. During the extraction, the inside of the vacuum pump needed to be humidified to avoid water loss in the working solution during the extraction. After the extraction was completed, the mold was put on a stereoscope to observe. If there were a few air bubbles at the edge, they could be picked out manually with a pipette. If there were more residual air bubbles, it was necessary to continue vacuumizing until the working solution filled the needle tip, and the excess working solution was recovered.
Step IV: the backing working solution was added into the PDMS concave mold, such that the backing solution covered and protruded the mold surface to form an arc, so as to avoid backing defects caused by water loss during the curing. The mold was dried and cured for 24 h at 20° C. and 15% air humidity for molding. The microneedle patch encapsulating the nucleic acid drug and photothermal nanoparticles was peeled off with tweezers or adhesive tape, as shown in
Regarding the drug delivery system, the example of the present disclosure further provided a use method of the drug delivery system, as shown in
Infrared laser light source irradiation was conducted to heat the photothermal nanoparticles in the microneedle patch. The photothermal nanoparticles conducted heat to the cell membrane, causing local arrangement of the cell membrane to be disordered, thereby allowing the drug to enter the cells.
As shown in the molecular dynamics simulation experiment results of
According to the research of the present disclosure, it was found that when the administration site was maintained at 50° C. to 80° C., the nucleic acid drug could quickly enter the cell membrane without causing damage to the cells.
1. Combining the mouse experiment shown in
2. At the end of this experiment, data collection was required, first of all, observation was conducted with a small animal fluorescence imager. After the end of experiment, the mice were observed at 24 h and 48 h once separately. The experimental mice were anesthetized with isoflurane before use. The software was started, and relevant settings were adjusted. A wavelength of the excitation light was set to 480 nm, a wavelength of the emitted light was set to 520 nm, and an exposure time was adjusted as needed; in this experiment, the exposure time was set to 200 s; the Binning was set to 2, the Fstop was set to 2, and then data were collected after photographing. The results were shown in
It is apparent that the above embodiments are merely listed for clear description, and are not intended to limit the implementations. The person of ordinary skill in the art may make modifications or variations in other forms based on the above description. There are no need and no way to exhaust all the implementations. Obvious changes or variations made thereto shall still fall within the protection scope of the present disclosure.