NUCLEIC ACID APTAMER AS1411 MODIFIED DNA TETRAHEDRON AND PREPARATION METHOD THEREOF

Abstract

This invention discloses a nucleic acid aptamer AS1411 modified DNA tetrahedron. The preparation method includes the steps of (1) binding an AS1411 sequence to the 5′ terminal of any DNA single-strand in a DNA tetrahedron, synthesizing the DNA, dissolving obtained DNA powder with ddH2O; (2) measuring an absorbance of the DNA and then calculating a total volume of the four single strands; (3) pipetting the DNA obtained in step (1) according to the calculation results in step (2), mixing the DNA with a TM buffer, mixing the mixture uniformly with vortex vibration, and performing a PCR progress. The preparation method is simple. The produced product can effectively solve the problem that the unmodified DNA tetrahedron cannot enter the nucleus and the problem that the AS1411 cannot carry drugs directly.

Description

CROSS REFERENCE TO RELATED APPLICATIONS

This application is the national phase entry of International Application No. PCT/CN2016/107816, filed on Nov. 30, 2016, which is based upon and claims priority to Chinese Patent Application No. CN201610942153.7, filed on Nov. 2, 2016, the entire contents of which are incorporated herein by reference.

TECHNICAL FIELD

The invention relates to the field of DNA tetrahedron, specifically to a nucleic acid aptamer AS1411 modified DNA tetrahedron and the preparation method thereof.

BACKGROUND

At present, the DNA tetrahedron has a great potential in the fields of medicine delivery, cancer treatment, etc., due to DNA tetrahedron's good biocompatibility, good stability and modifiability, and relatively simple synthesis method. The DNA tetrahedron can be used as a nano drug delivery with good biocompatibility. Compared to most traditional nano materials, DNA tetrahedron can be transported to cell lysosomes through caveolin-mediated endocytosis pathway mechanism, microtubule-dependent pathway, and can maintain the structure in cells for a relatively long time. DNA tetrahedron can successfully transport the immunostimulant CpG into cells to take effect. However, as with the individual DNA tetrahedron, the carried drugs also enter the lysosomes, which lead to the rapid degradation of drugs by lysosomes.

Nucleic acid aptamer AS1411 is a DNA single-strand that can specifically bind to pyrenin. Pyrenin is highly expressed on nucleus and the surface of the tumor cell membrane. Moreover, the AS1411 can enter the nucleus via the intracellular shuttle effect of the pyrenin. Meanwhile, the AS1411 can inhibit the DNA replication, so as to force the cells to stay in S phase, thereby inhibiting cell proliferation. AS1411 interferes with the binding of pyrenin and bcl-2 so as to promote apoptosis of cells. Hence, AS1411 has a great prospect in cancer diagnosis and treatment.

However, using the AS1411 nucleic acid aptamer to modify the DNA tetrahedron has not been reported yet.

SUMMARY OF THE INVENTION

In view of the above deficiencies in the prior art, this invention provides a nucleic acid aptamer AS1411 modified DNA tetrahedron and preparation method thereof. The present invention can effectively solve the problem that the unmodified DNA tetrahedron cannot enter the nucleus and the problem that the AS1411 cannot carry drugs directly.

In order to achieve the above objective, the technical solutions of this invention to solve the technical problem are as below:

A method for preparing a nucleic acid aptamer AS1411 modified DNA tetrahedron, including the following steps:

• • (1) binding an AS1411 sequence to any DNA single-strand of a DNA tetrahedron at the 5′ terminal of the DNA, synthesizing the DNA, centrifuging the obtained DNA powder at a high speed to ensure that the DNA powder aggregates at a bottom of the tube, dissolving the obtained DNA powder with ddH₂O, storing at the condition of 4° C.;
  • (2) measuring an absorbance of the DNA at wavelengths of 260 nm and 330 nm by ultraviolet quantitation method, then calculating the volume of each single strand in a 100 μL, 1 μM system according to the following formula:

V=100/[(A₂₆₀−A₃₃₀)×10⁵/(15.2×a number of adenine in a single strand+7.4×a number of cytosine in the single strand+11.4×a number of guanine in the single strand+8.3×a number of thymine in the single strand)],

• • calculating a total volume of the four single strands according to the above calculation results;
  • (3) pipetting the DNA obtained in step (1) according to the calculated total volume in step (2), mixing the DNA with a TM buffer to obtain a mixture, mixing the mixture uniformly with vortex vibration, and putting the mixture into a PCR apparatus; raising the temperature to 95° C. quickly and maintaining for 10 min; and then cooling down to 4° C. and maintaining for 20 min, and finally storing at −20° C. to obtain the nucleic acid aptamer AS1411 modified DNA tetrahedron.

Further, in step (1), 1 nmol DNA is dissolved in 10 μL ddH₂O.

Further, the TM buffer in step (3) having a pH value of 8.0 includes 5-10 mM Tris-HCl and 5-50 mM MgCl₂.

Further, the TM buffer in step (3) having a pH value of 8.0 includes 10 mM Tris-HCl and 50 mM MgCl₂.

The sequences of four DNA single strands of the DNA tetrahedron respectively are as below:

S1:
(SEQ ID NO: 1)
5′-ATTTATCACCCGCCATAGTAGACGTATCACCAGGCAGTTGAGACGA
ACATTCCTAAGTCTGAA-3′;
S2:
(SEQ ID NO: 2)
5′-ACATGCGAGGGTCCAATACCGACGATTACAGCTTGCTACACGATTC
AGACTTAGGAATGTTCG-3′;
S3:
(SEQ ID NO: 3)
5′-ACTACTATGGCGGGTGATAAAACGTGTAGCAAGCTGTAATCGACGG
GAAGAGCATGCCCATCC-3′
S4:
(SEQ ID NO: 4)
5′-ACGGTATTGGACCCTCGCATGACTCAACTGCCTGGTGATACGAGGA
TGGGCATGCTCTTCCCG-3′.

The AS1411 has a sequence of:

(SEQ ID NO: 5)
5′-GGTGGTGGTGGTTGTGGTGGTGGTGGT-3′.

The AS1411 can bind to any single strand of the DNA tetrahedron at the 5′ terminal of the DNA. The sequence thereof after binding is:

S1-AS1411:
(SEQ ID NO: 6)
5′-GGTGGTGGTGGTTGTGGTGGTGGTGGT-ATTTATCACCCGCCATA
GTAGACGTATCACCAGGCAGTTGAGACGAACATTCCTAAGTCTGAA-3′;
S2-AS1411:
(SEQ ID NO: 7)
5′-GGTGGTGGTGGTTGTGGTGGTGGTGGT-ACATGCGAGGGTCCAATA
CCGACGATTACAGCTTGCTACACGATTCAGACTTAGGAATGTTCG-3′;
S3-AS1411:
(SEQ ID NO: 8)
5′-GGTGGTGGTGGTTGTGGTGGTGGTGGT-ACTACTATGGCGGGTGA
TAAAACGTGTAGCAAGCTGTAATCGACGGGAAGAGCATGCCCATCC-3′;
S4-AS1411:
(SEQ ID NO: 9)
5′-GGTGGTGGTGGTTGTGGTGGTGGTGGT-ACGGTATTGGACCCTCGC
ATGACTCAACTGCCTGGTGATACGAGGATGGGCATGCTCTTCCCG-3′.

The verification of the nucleic acid aptamer AS1411 modified DNA tetrahedron: a polyacrylamide gel electrophoresis (PAGE) method is used. That is, diluting each of the unmodified single strand of the DNA tetrahedron by 100-fold, taking 5 μL of the dilution to mix with 1 μL of 6×loading buffer, taking 5 μL of the modified DNA tetrahedron to mix with 1 μL of 6×loading buffer, adding the solutions into a prepared gel (the ingredients of the gel: ultrapure water 4.2 mL, 40% acrylamide 1.2 mL, 10×TAE 0.6 mL, 10% APS 60 μL and TEMED 6 μL) respectively, adding a 20 bp marker in a side of the gel as a control, conducting electrophoresis in a 1×TAE buffer at a constant voltage of 100V for 80 minutes. Adding 50 ml ddH₂O and 5 μL Gel-red to a box without light, mixing uniformly, putting the gel into the box, shaking in a shaker for 15-20 minutes, and taking a picture via a gel imaging system.

The nucleic acid aptamer AS1411 modified DNA tetrahedron provided by the present invention has the following beneficial effects:

• • (4) The traditional DNA tetrahedron can only enter the cell but not the nucleus, and the AS1411 cannot deliver drugs directly. The present invention modifies the DNA tetrahedron with the nucleic acid aptamer AS1411 to form a drug carrier with high efficiency.
  • (5) The synthesis method is simple. The nucleic acid aptamer AS1411 can mediate the DNA tetrahedron into the nucleus to effectively improve the efficiency of drug delivery. The traditional DNA tetrahedron cannot enter the nucleus. Most of the cancer treating drugs inhibit biological behaviors of the tumor cells including proliferation and migration through binding to DNA, while most of the DNA exists in the nucleus. Thus, the AS1411 improves the efficiency of drug delivery by mediating the DNA tetrahedron onto the nucleus. Furthermore, the AS1411 itself can also inhibit the proliferation of tumor cells, and it can achieve double anti-tumor effect after delivering drugs.
  • (6) AS1411 can bind to pyrenin on the surface of tumor cell membrane in a targeted manner, whereas there is no pyrenin receptor on the surface of normal cells membrane. Therefore, the tetrahedron modified with AS1411 can deliver antitumor drugs in a targeted manner, such that the drug entering the tumor cells is significantly more than that entering the normal cells. Thus, the tumor cells can be treated well. Meanwhile, the damage to normal cells caused by the drug can be further reduced.

BRIEF DESCRIPTION OF THE DRAWINGS

Figure is an electrophoretogram of the nucleic acid aptamer AS1411 modified DNA tetrahedrons; wherein from right to left, the brands respectively are: marker, single strand S1, single strand S2, single strand S3, single strand S4, the nucleic acid aptamer AS1411 modified single strand S4, and the nucleic acid aptamer AS1411 modified DNA tetrahedron (Embodiment 4).

DETAILED DESCRIPTION OF THE INVENTION

Embodiment 1

A method for preparing a nucleic acid aptamer AS1411 modified DNA tetrahedron includes the following steps:

• • (4) binding an AS1411 sequence to S1 of the DNA tetrahedron at the 5′ terminal, synthesizing the DNA using an automatic DNA synthesizer to obtain a DNA powder, centrifuging the obtained DNA powder at a high speed to ensure that the DNA powder aggregates at a bottom of the tube, dissolving the obtained DNA powder with ddH₂O (1 nmol DNA is dissolved in 10 μL ddH₂O), storing at the condition of 4° C.;
  • (5) measuring an absorbance of the DNA at wavelengths of 260 nm and 330 nm by ultraviolet quantitation method, then calculating the volume of each single strand in a 100 μL, 1 μM system according to the following formula:

V=100/[(A₂₆₀−A₃₃₀)×10⁵/(15.2×a number of adenine in a single strand+7.4×a number of cytosine in the single strand+11.4×a number of guanine in the single strand+8.3×a number of thymine in the single strand)],

• • calculating a total volume of the four single strands according to the above calculation results;
  • (6) pipetting the DNA obtained in step (1) according to the calculated total volume in step (2), mixing the DNA with a TM buffer (10 mM Tris-HCl, 50 mM MgCl₂, pH 8.0) to obtain a mixture, mixing the mixture uniformly with vortex vibration, and putting the mixture into a PCR apparatus; raising the temperature to 95° C. quickly and maintaining for 10 min; and then cooling down to 4° C. and maintaining for 20min, and finally storing at −20° C. to obtain the nucleic acid aptamer AS1411 modified DNA tetrahedron.

Embodiment 2

A method for preparing a nucleic acid aptamer AS1411 modified DNA tetrahedron includes the following steps:

• • (4) binding an AS1411 sequence to S2 of the DNA tetrahedron at the 5′ terminal, synthesizing the DNA using an automatic DNA synthesizer to obtain a DNA powder, centrifuging the obtained DNA powder at a high speed to ensure that the DNA powder aggregates at a bottom of the tube, dissolving the obtained DNA powder with ddH₂O (1 nmol DNA is dissolved in 10 μL ddH₂O), storing at the condition of 4° C.;
  • (5) measuring an absorbance of the DNA at wavelengths of 260 nm and 330 nm by ultraviolet quantitation method, then calculating the volume of each single strand in a 100 μL, 1 μM system according to the following formula:

V=100/[(A₂₆₀−A₃₃₀)×10⁵/(15.2×a number of adenine in a single strand+7.4×a number of cytosine in the single strand+11.4×a number of guanine in the single strand+8.3×a number of thymine in the single strand)],

• • calculating a total volume of the four single strands according to the above calculation results;
  • (6) pipetting the DNA obtained in step (1) according to the calculated total volume in step (2), mixing the DNA with a TM buffer (10 mM Tris-HCl, 50 mM MgCl₂, pH 8.0) to obtain a mixture, mixing the mixture uniformly with vortex vibration, and putting the mixture into a PCR apparatus; raising the temperature to 95° C. quickly and maintaining for 10 min; and then cooling down to 4° C. and maintaining for 20 min, and finally storing at −20° C. to obtain the nucleic acid aptamer AS1411 modified DNA tetrahedron.

Embodiment 3

A method for preparing a nucleic acid aptamer AS1411 modified DNA tetrahedron includes the following steps:

• • (4) binding an AS1411 sequence to S3 of the DNA tetrahedron at the 5′ terminal, synthesizing the DNA using an automatic DNA synthesizer to obtain a DNA powder, centrifuging the obtained DNA powder at a high speed to ensure that the DNA powder aggregates at a bottom of the tube, dissolving the obtained DNA powder with ddH₂O (1 nmol DNA is dissolved in 10 μL ddH₂O), storing at the condition of 4° C.;
  • (5) measuring an absorbance of the DNA at wavelengths of 260 nm and 330 nm by ultraviolet quantitation method, then calculating the volume of each single strand in a 100 μL, 1 μM system according to the following formula:

V=100/[(A₂₆₀−A₃₃₀)×10⁵/(15.2×a number of adenine in a single strand+7.4×a number of cytosine in the single strand+11.4×a number of guanine in the single strand+8.3×a number of thymine in the single strand)],

• • calculating a total volume of the four single strands according to the above calculation results;
  • (6) pipetting the DNA obtained in step (1) according to the calculated total volume in step (2), mixing the DNA with a TM buffer (10 mM Tris-HCl, 50 mM MgCl₂, pH 8.0) to obtain a mixture, mixing the mixture uniformly with vortex vibration, and putting the mixture into a PCR apparatus; raising the temperature to 95° C. quickly and maintaining for 10 min; and then cooling down to 4° C. and maintaining for 20 min, and finally storing at −20° C. to obtain the nucleic acid aptamer AS1411 modified DNA tetrahedron.

Embodiment 4

A method for preparing a nucleic acid aptamer AS1411 modified DNA tetrahedron includes the following steps:

• • (4) binding an AS1411 sequence to S4 of the DNA tetrahedron at the 5′ terminal, synthesizing the DNA using an automatic DNA synthesizer to obtain a DNA powder, centrifuging the obtained DNA powder at a high speed to ensure that the DNA powder aggregates at a bottom of the tube, dissolving the obtained DNA powder with ddH₂O (1 nmol DNA is dissolved in 10 μL ddH₂O), storing at the condition of 4° C.;
  • (5) measuring an absorbance of the DNA at wavelengths of 260 nm and 330 nm by ultraviolet quantitation method, then calculating the volume of each single strand in a 100 μL, 1 μM system according to the following formula:

V=100/[(A₂₆₀−A₃₃₀)×10⁵/(15.2×a number of adenine in a single strand+7.4×a number of cytosine in the single strand+11.4×a number of guanine in the single strand+8.3×a number of thymine in the single strand)],

• • calculating a total volume of the four single strands according to the above calculated results;
  • (6) pipetting the DNA obtained in step (1) according to the calculated total volume in step (2), mixing the DNA with a TM buffer (10 mM Tris-HCl, 50 mM MgCl₂, pH 8.0) to obtain a mixture, mixing the mixture uniformly with vortex vibration, and putting the mixture into a PCR apparatus; raising the temperature to 95° C. quickly and maintaining for 10 min; and then cooling down to 4° C. and maintaining for 20 min, and finally storing at −20° C. to obtain the nucleic acid aptamer AS1411 modified DNA tetrahedron.

Verification of the nucleic acid aptamer AS1411 modified DNA tetrahedrons obtained by the above methods: a polyacrylamide gel electrophoresis (PAGE) method is used. That is, diluting each of the unmodified single strand of the DNA tetrahedron by 100-fold, taking 5 μL of the dilution to mix with 1 μL of 6×loading buffer, taking 5 μL of the modified DNA tetrahedron to mix with 1 μL of 6×loading buffer, adding the solutions into a prepared gel (the ingredients of the gel: ultrapure water 4.2 mL, 40% acrylamide 1.2 mL, 10×TAE 0.6 mL, 10% APS 60 μL, and TEMED 6 μL) respectively, adding a 20 bp marker in a side of the gel as a control, conducting electrophoresis in a 1×TAE buffer at a constant voltage of 100V for 80 minutes. Adding 50 ml ddH₂O and 5 μL Gel-red to a box without light, mixing uniformly, putting the gel into the box, shaking in a shaker for 15-20 minutes, and taking a picture via a gel imaging system. The electrophoretogram is shown in Figure.

Embodiment 6

20 mM pH 7.0 sodium phosphate buffer, 150 mM sodium chloride buffer, and 0.5 mM EDTA buffer are taken to prepare the following reaction system: 20 μM of the nucleic acid aptamer AS1411 modified DNA tetrahedron obtained in Embodiment 4, 400 μM of Adriamycin, 0.37% vol formaldehyde. The above reaction system is kept at 10° C. to react for 12 h. The obtained product using HPLC, molecular sieve, or ethanol precipitation method (the nucleic acid aptamer AS1411 modified DNA tetrahedron obtained in the present invention binding with drugs is referred as a sample, and the nucleic acid aptamer AS1411 modified DNA tetrahedron obtained without binding drugs is referred as a control) is purified.

The specificity and affinity of the samples against tumor cells are studied by flow cytometry. That is, the samples and the control (200 nM respectively) with tumor cells (A549) are incubated on the ice for half an hour respectively. The substance nonspecifically adsorbed on the cells is washed out with a DPBS buffer. The obtained cells are resuspended in a DPBS (including 5 mM Mg²⁺), and are analyzed using flow cytometry. The result shows that compared with the control, the samples have a specific recognition ability and higher affinity with respect to tumor cells.

Embodiment 7

Plating the cultured tumor cells A549 in 96-well cell culture plates (100 μL, 5×10⁴ cell/well), adding pure Adriamycin or samples with predetermined concentrations (0, 0.1 μM, 0.2 μM, 0.4 μM, 0.8 μM, 1.6 μM, 3.2 μM) into the wells respectively, culturing in a cell incubator for 1.5 h, centrifuging, removing the cell culture medium in the supernatant, adding fresh culture medium to continue culturing for 48 h, then testing the proliferation rate of the cells using a MTS reagent.

The testing result shows that, as the concentration increases, the proliferation rate of tumor cells decreases gradually, indicating that the inhibitory effect of the Adriamycin and samples against tumor cells increases gradually. Compared with the pure Adriamycin, the samples have a stronger inhibitory effect.

Claims

1. A method for preparing a nucleic acid aptamer AS1411 modified DNA tetrahedron, comprising the following steps: (1) binding an AS1411 sequence to any DNA single-strand of a DNA tetrahedron at the 5′ terminal of the DNA, synthesizing the DNA, dissolving the obtained DNA powder with ddH2O, storing at a condition of 4° C.;(2) measuring an absorbance of the DNA at wavelengths of 260 nm and 330 nm by ultraviolet quantitation method, then calculating a volume of each single strand in a 100 μL, 1 μM system according to the following formula: V=100/[(A260−A330)×105/(15.2×a number of adenine in a single strand+7.4×a number of cytosine in the single strand+11.4×a number of guanine in the single strand+8.3×a number of thymine in the single strand)],calculating a total volume of the four single strands according to the above calculated results of each single strand;(3) pipetting the DNA obtained in step (1) according to the calculated results in step (2), mixing the DNA with a TM buffer to obtain a mixture, mixing the mixture uniformly with vortex vibration, and putting the mixture into a PCR apparatus; raising the temperature to 95° C. quickly and maintaining for 10 min; and then cooling down to 4° C. and maintaining for 20min, and finally storing at -20° C. to obtain the nucleic acid aptamer AS1411 modified DNA tetrahedron.

2. The method for preparing a nucleic acid aptamer AS1411 modified DNA tetrahedron of claim 1, wherein in step (1), the DNA powder is dissolved in 10 μL ddH2O.

3. The method for preparing a nucleic acid aptamer AS1411 modified DNA tetrahedron of claim 1, wherein the TM buffer in step (3) having a pH value of 8.0 includes 5-10 mM Tris-HCl and 5-50 mM MgCl2.

4. The method for preparing a nucleic acid aptamer AS1411 modified DNA tetrahedron of claim 1, wherein the TM buffer in step (3) having a pH value of 8.0 includes 10 mM Tris-HCl and 50 mM MgCl2.

5. A nucleic acid aptamer AS1411 modified DNA tetrahedron, wherein the modified DNA tetrahedron is prepared through a method including the following steps: (1) binding an AS1411 sequence to any DNA single-strand of a DNA tetrahedron at the 5′ terminal of the DNA, synthesizing the DNA, dissolving the obtained DNA powder with ddH2O, storing at a condition of 4° C.;(2) measuring an absorbance of the DNA at wavelengths of 260 nm and 330 nm by ultraviolet quantitation method, then calculating a volume of each single strand in a 100 μL, 1 μM system according to the following formula: V=100/[(A260−A330)×105/(15.2×a number of adenine in a single strand+7.4×a number of cytosine in the single strand+11.4×a number of guanine in the single strand+8.3×a number of thymine in the single strand)],calculating a total volume of the four single strands according to the above calculated results of each single strand;(3) pipetting the DNA obtained in step (1) according to the calculated results in step (2), mixing the DNA with a TM buffer to obtain a mixture, mixing the mixture uniformly with vortex vibration, and putting the mixture into a PCR apparatus; raising the temperature to 95° C. quickly and maintaining for 10 min; and then cooling down to 4° C. and maintaining for 20 min, and finally storing at −20° C. to obtain the nucleic acid aptamer AS1411 modified DNA tetrahedron.

6. The nucleic acid aptamer AS1411 modified DNA tetrahedron of claim 5, wherein in step (1), the DNA powder is dissolved in 10 μL ddH2O.

7. The nucleic acid aptamer AS1411 modified DNA tetrahedron of claim 5, wherein the TM buffer in step (3) having a pH value of 8.0 includes 5-10 mM Tris-HCl and 5-50 mM MgCl2.

8. The nucleic acid aptamer AS1411 modified DNA tetrahedron of claim 5, wherein the TM buffer in step (3) having a pH value of 8.0 includes 10 mM Tris-HCl and 50 mM MgCl2.