CN103893755A - DNA-chitosan composite nano-particle, and preparation method and application thereof - Google Patents

DNA-chitosan composite nano-particle, and preparation method and application thereof Download PDF

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CN103893755A
CN103893755A CN201210575800.7A CN201210575800A CN103893755A CN 103893755 A CN103893755 A CN 103893755A CN 201210575800 A CN201210575800 A CN 201210575800A CN 103893755 A CN103893755 A CN 103893755A
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particle
nano
chitosan
dna
sequence
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万晓春
田永帅
马轶凡
蔡林涛
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Shenzhen Institute of Advanced Technology of CAS
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Abstract

The invention discloses a DNA/chitosan composite nano-particle. The DNA/chitosan composite nano-particle is a recombinant plasmid wrapped by a chitosan solubilization derivative and containing an AS2 short hairpin sequence, and the AS2 short hairpin sequence is a DNA sequence connected through a cyclic sequence and corresponding to siRNA of IL-10 gene. The invention also discloses a preparation method of the nano-particle, and an application of the nano-particle as an immunologic adjuvant. The nano-particle immunologic adjuvant has a good particle uniformity, can initiate cell immunostimulation, has small cytotoxicity and can rapidly and effectively inhibit the expression of interleukin-10 anti-inflammatory factors in order to realize the auxiliary enhancement of the effectiveness of vaccines; and the use of a chitosan nano-encapsulation technology realizes a sustained release effect in cells, and enables DNA to be degraded by endonucleases in histocytes.

Description

DNA-chitosan composite nanometer particle, its preparation and application
[technical field]
The present invention relates to immunologic adjuvant, be specifically related to a kind of DNA-chitosan composite nanometer particle, its preparation method, and apply as immunological adjuvant.
[background technology]
The new generation vaccine of continually developing out at present has good antigenic specificity and hypotoxicity, but vaccine immunogenicity is poor.Although successfully prepare the antigen getting a good chance of, can not induce enough strong preventive effect.For example, the Immunestimulatory effect of solubility protein purification vaccine or protein subunit vaccine conventionally a little less than, be not enough to stimulate body to produce enough antibody; While application separately, required antigen amount is more, and the antibody amount that body produces is less; And also easily cause immunologic tolerance.But these vaccines are when mating adjuvant and be used in conjunction, and above shortcoming will make moderate progress.Therefore develop immunological adjuvant safely and effectively and assist enhancing vaccine potency, significant for more new generation vaccines successful Application clinically.
The model of action of adjuvant is varied, and people are also abundant gradually to the knowledge of itself and immune system interphase interaction, and become modern immunologic important component part.Be engaged in respectively adjuvant research, understand adjuvant effect mechanism and Organism immunoregulation mode highly significant for deep.
Immunological adjuvant can be assisted a ruler in governing a country immunogen stimulates that body produces early, stronger, lasting immunne response.Desirable immunological adjuvant should be able to meet the following conditions: (1) is nontoxic or toxicity is minimum in effective dose; (2) can stimulate body to produce powerful humoral immunization and/or cellullar immunologic response; (3) there is lasting immunity; (4) do not induce autoimmune; (5) without mutagenesis, the effect of carcinogenic, teratogenesis shape etc.Although existing many adjuvants are applied to animal now, also do not have any adjuvant can meet above requirement completely.
In recent years, along with the 2nd, 3 generation the developing rapidly of vaccine, the very big development space that particularly polypeptide vaccine presents, impels immunological adjuvant also to have significant progress.
The adjuvant aluminium glue adjuvant that can be used for people of ratifying by FDA is at present deposited major defect both ways: one, can only produce humoral immunization by excitating organism, and can not inducing cell immunity.And cellular immunization is particularly necessary to the generation of body cell endoparasitism pathogen (virus, protozoon etc.) and tumour immunity power.Its two, aluminium glue adjuvant is to human immunodeficiency virus (HIV), hepatitis C virus (HCV), herpes simplex virus (HSV), influenza virus, and the antigen such as schistosomicide, pertussis and typhoid fever does not have adjuvanticity effect.Therefore can not meet the requirement of new generation vaccine development far away.
Nanotechnology is an emerging technology with bright prospects, and product-nanometer adjuvant that nanotechnology combines with immunological technique has become the focus of current vaccine research.From immunology viewpoint, nanometer adjuvant good uniformity, the antigen particles of parcel or the absorption just first-selection of macrophage (M5) and dendritic cell (DC) is engulfed target, and this is to realize the effective immunoreation of body to have completed an important step.And after nanometer adjuvant is connected with polypeptide antigen or DNA vaccination, can avoid the generation of conventional adjuvant carrier effect, play the effect of protection antigen.
[summary of the invention]
The present invention is intended to overcome the above defect of prior art, and the immunological adjuvant of Novel DNA-chitosan composite nanometer particle is provided.
Particularly, one aspect of the present invention provides a kind of DNA-chitosan composite nanometer particle, for the recombiant plasmid that contains the short hairpin of AS2 of chitosan solubilising derivant parcel, the short hairpin of described AS2 is sequence shown in the SEQNO.1 connecting by ring-shaped sequence and its complementary series.
Described chitosan solubilising derivant can be chitosan-polymine-polyethylene glycol polymer.
Described ring-shaped sequence can be TCAAGAG sequence.
The size of described recombiant plasmid can be 4610bp.
The particle diameter of described nano-particle can be 35-50nm.
The coated ratio of described chitosan solubilising derivant and described recombiant plasmid can be mol ratio 20:1.
The present invention is provided for preparing the method for this nano-particle on the other hand, comprises the following steps:
S1 synthesizes the short hairpin of AS2, and annealing;
S2 will be connected in buffer and mix with double digestion linear plasmid, DNA ligase through the short hairpin of AS2 of annealing, and transformed competence colibacillus escherichia coli, are inoculated in the LB culture medium containing ammonia benzyl resistance, do resistance examination, choose resistance bacterium colony, obtain recombiant plasmid solution; And
S3 mixes chitosan derivative solution with recombiant plasmid solution, obtain DNA-chitosan composite nanometer particle solution.
In step S3, the pH of chitosan solubilising derivative solution can be 5.5.
In step S3 chitosan solubilising derivative solution with recombiant plasmid solution before mixing, can be respectively at 65 DEG C of constant temperature 5 minutes.
Further aspect of the present invention provides the application of this nano-particle as immunological adjuvant.
Nano-particle immunological adjuvant good uniformity of the present invention; Can inducing cell immunity; Cytotoxicity is little; Can fast and effeciently reduce the expression that presses down scorching factor IL-10; Comprise technology by nano-particle, in cell, there is slowly releasing effect, and can protect DNA to avoid being degraded by intracellular nucleic acid restriction endonuclease.
[brief description of the drawings]
Fig. 1 illustrates the detected through gel electrophoresis result according to the recombiant plasmid of the embodiment of the present invention.
Fig. 2 is according to the scanning electron microscope image of the nano-particle of the embodiment of the present invention.
Fig. 3 illustrates the gel blocking electrophoresis detection result according to the nano-particle of the embodiment of the present invention.
Fig. 4 illustrates that nano-particle of the present invention is reducing the effect pressing down in scorching factor IL-10 expression.
[detailed description of the invention]
The cytokine of the initial a kind of uniqueness of finding the Th2 emiocytosis that is Mus of IL-10, found that B cell, Monocytes/Macrophages, keratinocyte and kinds of tumor cells and people's Th1 cell all can be secreted IL-10 afterwards.
IL-10 has very strong antiinflammatory and immunosuppressive activity, and it can suppress generation and the release of IL-2, IFN-C and proinflammatory factor; Can reduce immunity receptor MHC
Figure BDA00002656296400031
surface expression; Can suppress people's Th2 cell, cause the generation of hyperplasia and cytokine to reduce.
IL-10 has multiple inhibit feature, for example, suppress mononuclear cell dependent T h hyperplasia; Suppress the synthetic and active of Th1 class lymphokine; Suppress onthe surface of monocytes MHC
Figure BDA00002656296400032
quasi-molecule is expressed, and reduces monocytic HLA-II antigen, the generation of the blocking-up antigenic specificity Monocytes/Macrophages factor; The activity that suppresses NK cell, IL-10 does not directly act on NK cell, but indirectly plays a role by the generation that suppresses IFN-C.To NK cell proliferation, activation has Pasitive Regulation Effect of Genseng to IFN-C.The apoptosis of 1/4 suppressor T cell, isolated T cell from peripheral blood lymphocytes, as added IL-10 can reduce the apoptosis of T cell in culture fluid.The generation of inhibitory reaction nitrogen oxide, reactive nitrogen oxide is significant to parasitic removing inside and outside intracellular products and cell.
IL-10 has very strong immunostimulation, comprising: the propagation, the maturation that promote non-mononuclear cell dependent T cell.Under the condition existing at IL-3, IL-4, stimulate the propagation of mastocyte and CFU-GM thereof, strengthen the vigor of mastocyte.Stimulator antigen specific b cells propagation, and be divided into plasma cell.
Based on this, the inventor has designed the recombiant plasmid of the short hairpin of a kind of AS2 of including, and the short hairpin of this AS2 is sequence and its complementary series shown in the SEQ NO.1 connecting by ring-shaped sequence.
the design of the short hairpin of AS2
Obtain hIL-10 gene order by GeneBank, designed a RNAi target position for its 5 ' AUG district.Between complementary siRNA, introduce a circulus sequence, this ring-shaped sequence can be, for example TCAAGAG.Hold and introduce respectively BamH I and Hind III restriction enzyme site at shRNA5' end and 3', antisense fragment meets termination signal TTTTT later, transcribes stopping.So, formed the structure of BamH I+ positive-sense strand+loop chain+antisense strand+termination signal+Hind III.
The antisense dna sequence of the designed shRNA of chemosynthesis, i.e. AS2 sequence of the present invention.In contrast, the inventor also uses identical ring-shaped sequence TCAAGAG, connects sequence shown in SEQ NO.2, has synthesized control sequence (contrast).
In order to form stable DNA double chain, the synthetic DNA sequence obtaining is annealed.Dissolve respectively synthetic AS2 fragment (positive-sense strand and antisense strand) with sterilizing tri-distilled water and dissolve, final concentration is 10umol/L.And complete annealing by following condition: positive-sense strand 2uL, antisense strand 2uL, 10x annealing buffer 2ul, adding tri-distilled water is 20uL to cumulative volume, in 80 DEG C of water-baths 2 minutes, slowly cools to room temperature (16 DEG C), completes annealing.
recombiant plasmid
preparation:
For obtaining recombiant plasmid, the inventor has used pSilencer 3.1-H1 hygro carrier to build pS-AS2-IL10 expression vector.
First, utilize pSilencer 3.1-H1 hygro, obtain shape material grain: according to pSilencer 3.1-H1hygro carrier description, prepare plasmid solution 1ug/uL; Transformed competence colibacillus bacillus coli DH 5 alpha; Be inoculated in the LB solid medium of ampicillin (ampcillin); Resistance screening extracts plasmid pSilencer 3.1-H1; By BamH I and Hind III double digestion; Glue reclaims enzyme action product, obtains linear object plasmid 20uL(16ug/uL).
Afterwards, connect linear object plasmid and the DNA fragmentation through annealing.Double digestion linear plasmid pSilencer 3.1-H1 4uL, through annealing AS2 sequence 1uL, T4 DNA ligase 2uL, 10 times connect buffer (ligation buffer) 2uL, adding sterilizing tri-distilled water to cumulative volume is 20uL, in 16 DEG C of water-baths 12 hours, be placed in afterwards 65 DEG C of water-baths 10 minutes.Transformed competence colibacillus escherichia coli, are inoculated in the LB culture medium containing ammonia benzyl resistance, do resistance screening, choose resistance bacterium colony.Obtain recombiant plasmid (pS-AS2).
Use contrast DNA sequence, with identical method, index obtains control plasmid (pS-contrast).
characterize:
After resistance screening, get resistance bacterium colony, be bacterium colony PCR at the insertion point upstream and downstream design primer bacterium colony of recombiant plasmid and identify whether expanding fragment length is Insert Fragment length, primer is: 3.1sq-F:TCTTTGGATTTGGGAATCTTAT, 3.1sq-R:ACACAGGAAACAGCTATGA.Send the order-checking of Invitrogen company by the sizeable bacterium colony of PCR product fragment, further the correctness of qualification restructuring quality.
After bacterium colony PCR product electrophoresis detection, stripe size is Insert Fragment size, and Invitrogen company sequencing result shows that shRNA expresses correct being inserted in pSilencer3.1-H1 carrier of fragment.
Fig. 1 illustrates gel electrophoresis (1% agarose gel) testing result of this recombiant plasmid.Recombiant plasmid is prepared rear electrophoresis band and is shown that clip size is approximately 5000bp, and band brightness is higher, meets expection.
nano-particle
Further, the inventor combines this recombiant plasmid with nanotechnology, utilizes chitosan solubilising derivant parcel recombiant plasmid, to form nano-particle.
Chitosan is unique a kind of cationic polysaccharide that occurring in nature is found so far, and in aqueous solution, ionization is cation.The band polarity cationic nano-grain so forming, is convenient to be adsorbed onto on the cell membrane with negative charge, promotes the endocytosis of cell.So just can make the molecular medicine of chitosan nano particle packaging be convenient to by Cell uptake.And the biocompatibility of chitosan is very good, the nano-particle of preparing with it is very low to cytotoxicity, itself just can be used as a kind of immunostimulant and use, therefore pack with it, can to suppress the DNA molecular medicine that IL-10 expresses will be a kind of extraordinary immunostimulant, i.e. vaccine adjuvant.
But chitosan is poor because of water solublity, the use in organism also has certain limitation.The present invention uses through the chitosan solubilising derivant of modification, and for example chitosan-polymine-polyethylene glycol polymer (CS-N-PEI-PEG) has improved the water solublity of chitosan greatly.Its with cationic charge increase, its transfection efficiency is improved greatly.
In addition, because the molecular conformation of such chitosan derivatives is more complicated, the nano-particle preparing with it is to pack nano-particle molecule assembling after can making after DNA to pack tightr, in cell, can more effectively resist the shearing of cell DNA enzyme to foreign DNA, play the slow releasing function to IL-10 disturbing molecule.
preparation:
In the present invention, prepare the recombiant plasmid of chitosan solubilising derivant parcel with ionic cross-linking.By chitosan solubilising derivant CS-N-PEI-PEG(chitosan-polymine-polyethylene glycol polymer, with reference to " research of the preparation of Polyethylene Glycol-chitosan-polyethylene imine copolymer and gene delivery system performance thereof "--Zhongshan University's doctorate paper---Zhang Wei, Pan Shirong etc., 20080420, prepare) solution (pH5.5), recombiant plasmid solution, respectively at 65 DEG C of constant temperature water baths 5 minutes.Then the two is evenly mixed 10 minutes, obtain the nano-particle of chitosan solubilising derivant parcel recombiant plasmid, i.e. DNA-chitosan composite nanometer particle of the present invention (CNP-pS-AS2).
Use contrast DNA sequence, with identical method, obtain contrast nano-particle (CNP-pS-contrast).
characterize:
1. the form of nano-particle, particle diameter and Zeta potential are measured
The plasmid chitosan nano sample liquid that takes a morsel is observed nano-particle form and takes pictures under transmission electron microscope.Separately get nano-particle sample liquid appropriate, add distilled water dilution rear with Zetasizer3000HS/IHPL nano-particle size analysis instrument mensuration particle diameter, dispersion and Zeta potential.
Electromicroscopic photograph is shown in Fig. 2, and the electron microscopic observation result in figure shows that how spherical in shape chitosan nano particle is, and uniformity is better.
Nano-particle size analysis instrument measurement result is as shown in table 1 below:
The particle diameter of table 1 nano-particle and Zeta potential
Nano-particle Particle diameter (nm) Zeta potential (mV)
CNP-pS-AS2 42.1 129.0
CNP-pS-contrast 42.3 131.2
Nano-particle more little being more easily transfected in cell of particle diameter, transfection efficiency is higher, tube wall that can distributed by capillarity in the time that nano particle diameter is less than 80nm.So the particle diameter of granule of the present invention within the scope of 30-50nm, makes granule of the present invention can make injection or oral drugs, be beneficial to penetration rate of blood tube wall and enter blood circulation, be beneficial to drug delivery, be an extraordinary delivery system.
2. gel retardation assay
Get respectively pS-AS2 recombiant plasmid solution and CNP-pS-AS2 nano-particle sample liquid is carried out 0.7% agarose gel electrophoresis, to detect the parcel effect of nano-particle of the present invention.C is pSilencer 3.1-H1 empty carrier, and 2 is DNA-chitosan composite nanometer particle (CNP-pS-AS2).
0.7% agarose gel horizontal strip electrophoresis result is as shown in Figure 3: with compare, the recombiant plasmid of CS-N-PEI-PEG parcel loses band in 5000bp position, micro-in well have a bright spot.This explanation nucleic acid dye cannot be directly and DNA polymerization; Or the particle diameter of DNA-chitosan composite nanometer particle is excessive, and cannot pass through agarose polymeric aperture.Illustrate that DNA-chitosan composite nanometer particle wraps up successfully.
immunity test
to lymphocytic transfection:
In Tissue Culture Plate, add respectively DNA-chitosan composite nanometer particle of the present invention (CNP-pS-AS2), make its final concentration be 2ug/ml.Transfection is added hyclone in backward culture medium in 4 hours, and making serum final concentration is 10%.
the detection by quantitative of quantitative PCR gene involved in immunity
Expression analysis carries out with Bio-Rad iQ5 quantitative PCR instrument.Taking leukocyte cDNA as template, increase with listed primer in following table 2.Detect the variation of cytokine IL-10 expression, to illustrate whether immunological effect improves.
Table 2
Title Primer sequence (5 '-3')
IL-10-F CGGCGCTGTCATCAATTTCTG
IL-10-R CCCCTCTCTTGGAGCTTGCTA
β-actin-F CAGCTCCTCCCTGGAGAAGAGCTA
β-actin-R CTTCTGCATCCTGTCGGCAATGCC
Quantitative pcr amplification parameter is: 95 DEG C of denaturations 30 seconds; 95 DEG C 30 seconds; 60 DEG C 60 seconds; Circulate 45 times.
Solubility curve parameter is: 65-95 DEG C, rises 0.5 DEG C for every 10 seconds.
Using β-actin as reference gene, adopt Δ Δ Ct method to analyze real-time fluorescence quantitative PCR data, relative expression's level of more same genes of interest different times.
Fig. 4 is illustrated in to press down in scorching factor IL-10 and adds respectively DNA-chitosan composite nanometer particle of the present invention; The positive control Cp of the breeding of activated viral agent pig and breathing syndrome virus (PRRSV); And when not adding activated viral agent and also not adding nano-particle of the present invention (blank C), relative expression's level of IL-10.
From chart, after adding CNP-pS-AS2 of the present invention, the expression of IL-10 is obviously suppressed, and in 48 hours, suppression ratio is more than 95%.
It is a species specific PTGS mechanism that RNA disturbs (RNAi), and this is by the transcriptional control mechanism numerator mediated with the siRNA of 19-27 nucleotide of target gene homologous complementary.SiRNA and analog thereof can carry out reversibly inhibition of gene expression for pre-mRNA or ripe mRNA in vivo and in vitro specially, the regulation and control that realize IL-10 expression by RNAi technological means have feasibility, but its application is subject to the siRNA half-life short, is easy to the effects limit such as degraded.
The present invention designs the double chain DNA sequence of expressing shRNA, be building up in psilencer3.1-H1 carrier, being wrapped to form nano-particle by chitosan is transfected in cell, chitosan nano particle can stop the degraded of DNA to expression vector in cell, expression vector can continue to transcribe the shRNA forming for IL-10 in cell, thereby realizes the effect of the expression of the inhibition IL-10 gene of persistent high efficiency.
To sum up, the present invention passes through to use the AS2 sequence of unique design, and is reconstituted in after plasmid, is wrapped in chitosan, has obtained effectively suppressing fast the nano-particle that IL-10 expresses, thereby can be used as immunological adjuvant.
DNA-chitosan composite nanometer particle good uniformity of the present invention, mean diameter is 42.1nm, is distributed within the scope of 30nm-50nm, homogeneity is good, and nano-particle is with cationic charge, utilizes and is adsorbed onto cell surface, is conducive to be transfected in cell.
Nano grain surface, with positive charge (Zeta potential 129.0), is easy to merge with the cell membrane with negative charge, is convenient to dendritic cell and macrophage phagocytic, thus trigger cell immunostimulation;
Owing to having used chitosan parcel, nano-particle of the present invention has slowly releasing effect in cell, and can stop the degraded of the DNA of intracellular nucleic acid restriction endonuclease to nano-particle parcel.
The above the specific embodiment of the present invention, does not form limiting the scope of the present invention.Various other corresponding changes and distortion that any technical conceive according to the present invention has been done, all should be included in the protection domain of the claims in the present invention.
Figure IDA00002656297200011
Figure IDA00002656297200021
Figure IDA00002656297200031

Claims (10)

1. a DNA-chitosan composite nanometer particle, is the recombiant plasmid that contains the short hairpin of AS2 of chitosan solubilising derivant parcel, and the short hairpin of described AS2 is sequence and its complementary series shown in the SEQ NO.1 connecting by ring-shaped sequence.
2. nano-particle according to claim 1, is characterized in that, described chitosan solubilising derivant is chitosan-polymine-polyethylene glycol polymer.
3. nano-particle according to claim 1, is characterized in that, described ring-shaped sequence is TCAAGAG sequence.
4. nano-particle according to claim 1, is characterized in that, the size of described recombiant plasmid is 4610bp.
5. nano-particle according to claim 1, is characterized in that, the particle diameter of described nano-particle is 35-50nm.
6. nano-particle according to claim 1, is characterized in that, the coated ratio of described chitosan solubilising derivant and described recombiant plasmid is mol ratio 20:1.
7. for the preparation of the method for the nano-particle described in any one in claim 1-6, comprise the following steps:
S1 synthesizes the short hairpin of AS2, and annealing;
S2 will be connected in buffer and mix with double digestion linear plasmid, DNA ligase through the short hairpin of AS2 of annealing, and transformed competence colibacillus escherichia coli, are inoculated in the LB culture medium containing ammonia benzyl resistance, do resistance examination, choose resistance bacterium colony, obtain recombiant plasmid solution; And
S3 mixes chitosan solubilising derivative solution with recombiant plasmid solution, obtain DNA-chitosan composite nanometer particle solution.
8. method according to claim 7, is characterized in that, in step S3, the pH of chitosan solubilising derivative solution is 5.5.
9. method according to claim 7, is characterized in that, in step S3 chitosan solubilising derivative solution with recombiant plasmid solution before mixing, respectively at 65 DEG C of constant temperature 5 minutes.
In claim 1-6 the nano-particle described in any one as the application of immunological adjuvant.
CN201210575800.7A 2012-12-26 2012-12-26 DNA-chitosan composite nano-particle, and preparation method and application thereof Pending CN103893755A (en)

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Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN106337052A (en) * 2016-08-26 2017-01-18 南京大学 Antisense oligodeoxynucleotide and application thereof

Non-Patent Citations (4)

* Cited by examiner, † Cited by third party
Title
ARVIND CHHABRA ET AL.: "Silencing of Endogenous IL-10 in Human Dendritic Cells Leads to the Generation of an Improved CTL Response Against Human Melanoma Associated Antigenic Epitope, MART-1(27−35)", 《CLIN IMMUNOL.》 *
ARVIND CHHABRA ET AL.: "Silencing of Endogenous IL-10 in Human Dendritic Cells Leads to the Generation of an Improved CTL Response Against Human Melanoma Associated Antigenic Epitope, MART-1(27−35)", 《CLIN IMMUNOL.》, vol. 126, no. 3, 31 March 2008 (2008-03-31), pages 251 - 259, XP022477505, DOI: 10.1016/S0022-1139(97)00030-4 *
GRO FURSET, MOULDY SIOUD: "Design of bifunctional siRNAs: Combining immunostimulation and gene-silencing in one single siRNA molecule", 《BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS》 *
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* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN106337052A (en) * 2016-08-26 2017-01-18 南京大学 Antisense oligodeoxynucleotide and application thereof

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Application publication date: 20140702