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Soluble microneedle patch and preparation method thereof

A probe and chip technology, applied in the field of soluble microneedle patches and its preparation, can solve the problems of poor detection ability of mixed genotypes, HBsAg antigenic changes, and difficulty in detecting multi-gene locus mutations

Active Publication Date: 2018-04-20
302 MILITARY HOSPITAL OF CHINA
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  • Abstract
  • Description
  • Claims
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AI Technical Summary

Problems solved by technology

Mutations in the S gene region, especially the mutation at the amino acid 145 position of the "α" determinant, will lead to changes in the antigenicity of HBsAg, making it undetectable by the widely used HBsAg diagnostic reagents in clinical practice, resulting in missed detection, which may lead to Cause such virus carriers to become blood donors, bringing serious consequences to blood recipients
[0004] At present, there are four main molecular detection methods for HBsAg gene variation: (1) sequencing method: the gold standard for HBV gene detection, with high accuracy, but low sensitivity and long time-consuming; (2) RFLP method: the principle is to The DNA fragment to be tested is digested with a restriction endonuclease to identify and cut the specific sequence, and the digested product is subjected to electrophoresis to determine whether the target gene has a specific sequence according to the size of the DNA fragment, but the degree of standardization Low, poor ability to detect mixed genotypes. When detecting gene mutations, multiple detection systems are required to detect mutations of more than 1 base; (3) Quantitative PCR method: high sensitivity, but low throughput, It is difficult to detect multi-gene locus variation; (4) Reverse linear probe hybridization method: first point known probes on nitrocellulose membrane or nylon membrane respectively, and PCR amplification with 5' end-labeled biotin primers The product is hybridized, and then the hybridization signal is displayed by the corresponding color reaction
The naked eye interpretation is easy to misjudge, the detection cost is high, and it is difficult to carry out routinely in domestic clinical laboratories

Method used

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  • Soluble microneedle patch and preparation method thereof
  • Soluble microneedle patch and preparation method thereof
  • Soluble microneedle patch and preparation method thereof

Examples

Experimental program
Comparison scheme
Effect test

Embodiment 1

[0090] Embodiment 1, the preparation of gene chip

[0091] According to the characteristics of the prevalence of hepatitis B virus (HBV) sequences in my country, the oligonucleotide probes used to detect 4 HBsAg mutation sites are designed, as shown in Table 1 (the probes in Table 1 are all carried out at the 3' end. NH 2 modified).

[0092] The HBsAg wild type is shown in sequence 14 of the sequence listing. The four HBsAg mutation sites are: (1) S118: amino acid 118 of HBsAg; (2) S120: amino acid 120 of HBsAg; (3) S126: amino acid 126 of HBsAg; (4) S145: amino acid 145 of HBsAg bit amino acid.

[0093] Table 1 Probe information

[0094] probe name

Probe sequence (5'-3')

base number

118T19

CTACCAGCACGGGACMATGTTTTTTTTTTTT (sequence 1)

31

118K19

CTACCAGCAAGGGACMATGTTTTTTTTTTTT (sequence 2)

31

120P17

CAMGGGACCATGCAAAATTTTTTTTTTTT (sequence 3)

29

120Q17

CAMGGGACAATGCAAAATTTTTTTTTTTT (sequence 4)

29

126...

Embodiment 2

[0104] Embodiment 2, establishment of detection method

[0105] 1. Take the serum to be tested, and use the virus DNA out kit to extract the virus DNA according to the instructions.

[0106] 2. Using the viral DNA obtained in step 1 as a template, carry out a nested PCR reaction to obtain a PCR amplification product (about 1200bp);

[0107] Specific steps are as follows:

[0108] (1) The first round of PCR, reaction system: template (viral DNA) 5 μl, PCR reaction solution 12 μl, upstream and downstream primers 2.5 μl each, ddH 2 O 2.5 μl, Taq enzyme 0.5 μl; PCR reaction program: pre-denaturation at 94°C for 3 minutes, denaturation at 94°C for 35 s, annealing at 59°C for 35 s, extension at 72°C for 70 s, 2 cycles; denaturation at 94°C for 35 s, annealing at 57°C for 35 s, and 72°C Extension 70s, 2 cycles; denaturation at 94°C for 35s, annealing at 55°C for 35s, extension at 72°C for 70s, 2 cycles; denaturation at 94°C for 35s, annealing at 53°C for 35s, extension at 72°C for ...

Embodiment 3

[0126] Embodiment 3, clinical sample detection

[0127] Research objects: 40 patients with chronic hepatitis B, 24 males and 16 females, in line with the diagnosis of chronic hepatitis B in the Chinese Medical Association Hepatology Branch, Chinese Medical Association Infectious Diseases Branch: Guidelines for the Prevention and Treatment of Chronic Hepatitis B (2015 Edition) Criteria, excluding autoimmune diseases and other liver diseases.

[0128] Serum samples were taken from the research subjects and tested according to the method in Example 2.

[0129] The electrophoresis diagram of the PCR amplification product obtained in step 2 of some samples is shown in figure 2 , the size of the amplified product is about 1200bp, which is consistent with the expectation; the electropherogram of the PCR amplified product obtained after step 6 is shown in image 3 , the size of the amplified products is about 300bp, which is consistent with the expectation.

[0130] A total of 40 ...

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Abstract

The invention discloses a soluble microneedle patch and a preparation method thereof. The invention provides a whole set of probes which are composed of single-stranded DNA molecules as shown in sequence 1-9 in a sequence table. The invention also discloses a gene chip prepared by immobilizing the whole set of probes on a chip medium. The gene chip can be used for detecting the mutation of the HBsAg sites in to-be-detected samples. During detection, the DNAs of viruses are extracted from the serum samples of to-be-detected patients and then subjected to in-vitro amplification and hybridizationwith the probes in the chip, and the types of mutation can be determined according to hybridization signals. A detection method provided by the invention has the advantages of high throughput, high specificity, simple operation, automatic judgment of results and easy realization of standard control, is applicable to clinical detection of HBsAg gene mutation, and can meet the needs of physical examination and blood donor screening.

Description

technical field [0001] The invention relates to a dissolvable microneedle patch and a preparation method thereof. Background technique [0002] Hepatitis B is caused by infection with the hepatitis B virus (HBV). HBV belongs to the hepadnaviridae family and is a circular double-stranded DNA virus. The outer layer is a lipoprotein envelope containing hepatitis B surface antigen (HBsAg); the inner layer is a core containing nucleic acid and hepatitis B core antigen. [0003] The HBV S gene encodes surface antigen (HBsAg). HBsAg has important biological significance, is the main component of hepatitis B vaccine, and is an important basis for diagnosing hepatitis B virus infection. The S gene region can be divided into three segments: the S region, the pre-S1 region and the pre-S2 region. Each of the three segments has a start codon (AUG) at the 5' end, but shares a stop codon. The translated products form the major protein (226 amino acids), medium protein (281 amino acids) ...

Claims

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Application Information

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IPC IPC(8): C12Q1/6883C12Q1/6837C12N15/11
CPCC12Q1/6837C12Q1/6883C12Q2600/156
Inventor 钟彦伟张敏顾梅蕾谢进张秀昌杨艳杰赫兢
Owner 302 MILITARY HOSPITAL OF CHINA
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