• 한국동물생명공학회지
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• 제38권4호
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• pp.209-214
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• 2023

Background: Single nucleotide polymorphisms (SNPs) are widely used genetic markers with applications in human disease diagnostics, animal breeding, and evolutionary studies, but existing genotyping methods can be labor-intensive and costly. The aim of this study is to develop a simple and rapid method for identification of a single nucleotide change. Methods: A modified Polymerase Chain Reaction Amplification of Multiple Specific Alleles (PAMSA) and high resolution melt (HRM) analysis was performed to discriminate a bovine polymorphism in the NCAPG gene (rs109570900, 1326T > G). Results: The inclusion of tails in the primers enabled allele discrimination based on PCR product lengths, detected through agarose gel electrophoresis, successfully determining various genotypes, albeit with some time and labor intensity due to the use of relatively costly high-resolution agarose gels. Additionally, high-resolution melt (HRM) analysis with tailed primers effectively distinguished the GG genotype from the TT genotype in bovine muscle cell lines, offering a reliable way to distinguish SNP polymorphisms without the need for time-consuming AS-PCR. Conclusions: Our experiments demonstrated the importance of incorporating unique mismatched bases in the allele-specific primers to prevent cross-amplification by fragmented primers. This efficient and cost-effective method, as presented here, enables genotyping laboratories to analyze SNPs using standard real-time PCR.

• Journal of Microbiology
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• 제40권1호
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• pp.70-76
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• 2002

Proviral DNAs from HIV-1-infected CD4+ T cells (Molt/LAV cells) were amplified and detected in infected individual cells using polymerase chain reaction and in rifu hybridization. In this in situ PCR, three parameters were considered to achieve effective amplification and retention of amplificants inside the cells by making high molecular weight PCR products intracellularly, forming agarose matrix against the cells, and maintaining the appropriate PCR temperature profile. Over the cycles of ampliHcationl tailed primers with complementary overhanging sequences at their 5' sides manufactured high molecular weight products by using short primary products as a repeating unit. Agarose matrix could prevent the diffusion of the amplificants from the cells. Use of Thermanox coverslip inside the PCR tube offered target cells a similar temperature profile to that of conventional PCR in solution.

• 미생물학회지
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• 제40권2호
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• pp.167-171
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• 2004

효과적인 원위치 중합효소 연쇄반응 (In situ PCR)을 위해서는 증폭된 PCR 산물의 세포외 유출을 감소시켜야 한다. 이를 위한 한 방법으로 거대분자 PCR 산물을 합성시키기 위한 5'쪽에 서로 상보적인 꼬리서열을 가진 프라이머(꼬리 프라이머; tailed primer)가 사용되었으나 많은 PCR 횟수로 인해 시간의 낭비와 세포조직의 형태보존성이 저하되는 문제가 발생하였다. 따라서 PCR 조건을 가능한 최적화시키고, 최소의 PCR 횟수로써 세포외 유출을 막을 수 없는 방법이 필요하게 되었다. 이러한 방법의 일환으로 꼬리 프라이머를 이용하여 PCR 튜브 속에서 목표 핵산없이 프라이머 중합체(primer polymers)의 형성을 유도하였고, 이를 유리 슬라이드위에 고정시킨 Molt/LAV 세포들에 처리하여 20 회의 짧은 시간에서도 적절한 탐침을 할 수 있게 되었다. 이로 인해 프라이머 중합체의 원위치 중합효소 연쇄반응에서의 사용가능성을 타진하였다.

• BMB Reports
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• 제38권3호
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• pp.350-353
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• 2005

Alanine at residue 73 (Ala-73) and aspartate at residue 9 (Asp-9) are characteristic to both Cw6 and Cw7 alleles of HLA-C gene and have been suggested as possible markers for psoriasis vulgaris (PsV). However, the results from various ethnic groups/populations are contradictory and inconclusive. In this study, an attempt has been made to examine the association between HLA-C (Ala-73 and Asp-9) and susceptibility to PsV among Saudi patients. Genomic DNA was extracted from 25 Saudi PsV patients and 75 control subjects. Polymerase chain reaction (PCR) was performed to amplify HLA-C sequences using earlier reported primers, C133P and C243PR. Sequence-specific primers were used to specifically detect nucleotide coding for Ala-73 and Asp-9 in all the subjects. The results showed significantly higher frequency of Asp-9 (84.0% versus 61.3%) in PsV patients as compared to controls (p < 0.05, 2-tailed Fisher's exact test). The frequencies of Ala-73 among PsV patients (92%) and controls (88%) did not differ significantly.

• 미생물학회지
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• 제37권4호
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• pp.294-298
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• 2001

감염성 바이러스의 발생은 세계적인 현상으로 어린이는 물론 성인의 건강을 위협하고 있는 실정이다. 1998년 -2000년 사이에 부산지역 바이러스성 전염병 유행예측사업의 과정에서 소화기계 바이러스가 탐색되었다. 의심되는 환자의 대변 및 뇌척수액, 인후가검물에서 세포배양, Latex 응집반응, 간접면역형광항체법, 전자현미경 관찰 등을 행하여 바이러스를 확인하였다. 총 검체 중에서 바이러스의 확인 율은 12.5% 이었다. 이 과정을 통하여 3 사례의 장 adenovirus 및, 23 사례의 echovirus, 31 사례의 coxsackievirus, 36 사례의 rotavirus, 45 사례의 small round structured virus (SRSV), 7 사례의 poliovirus가 확인되었다. 확인된 주요 혈청형으로는 장 adenovirus 41형 및 echovirus 6, 9, 11, 25, 30형, coxsackievirus B2, B3, B4, B6 형 등이 탐색되었다. 각 바이러스의 월별 발생별로는 SRSV는 12월에서 다음해 4월 사이, echovirus와 coxsackievirus는 4월에서 10월 사이에, rotavirus는 1월에서 4월 사이에 각각 분리 율이 높았다. 전자현미경 관찰에서는 30-80 nm의 작은 크기의 바이러스들이 확인되었다.

• Asian-Australasian Journal of Animal Sciences
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• 제18권10호
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• pp.1375-1378
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• 2005

The objective of this study was to investigate polymorphisms of BMPRIB (bone morphogenetic protein type IB receptor) gene and its effect on litter size traits in sheep. Three populations including 101 Small Tailed Han sheep, 79 Poll Dorset and 81 hybrids (Poll Dorset${\times}$Small Tailed Han sheep) were used to detect the polymorphisms in exon 6 region of sheep BMPRIB gene. A fragment of approximately 190bp was amplified by one pair of primers, the polymorphism was revealed from the analysis of three populations by the technique of PCR -SSCP, and a mutation from A to G at 746 of the coding region was confirmed by sequencing in several individual. Statistical results indicated the distribution of allele B (with a A$\longrightarrow$G mutation) and A (without mutation) or genotype AA, AB and BB frequencies differed in three populations. BB genotype (44.55%) and B allele (66.34%) frequencies of Small Tailed Han sheep were higher than those of the others. Analysis of variance showed that the polymorphism of BMPRIB gene was associated with positive effect on litter size traits. The means of genotype BB and AB were about 1.04 and 0.74 more than genotype AA for litter size (p<0.05). Analysis of BMPRIB genotype effects on litter size in three populations indicates the existence of genotype BB or B allele increases the litter size. It suggested that the polymorphism in exon 6 (at 746 in the coding region) of sheep BMPRIB gene may be used as a marker for early selection of prolificacy in sheep.

• Asian-Australasian Journal of Animal Sciences
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• 제29권5호
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• pp.631-639
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• 2016

China has a long history of sheep (Ovis aries [O. aries]) breeding and an abundance of sheep genetic resources. Knowledge of the complete O. aries mitogenome should facilitate the study of the evolutionary history of the species. Therefore, the complete mitogenome of O. aries was sequenced and annotated. In order to characterize the mitogenomes of 3 Chinese sheep breeds (Altay sheep [AL], Shandong large-tailed sheep [SD], and small-tailed Hulun Buir sheep [sHL]), 19 sets of primers were employed to amplify contiguous, overlapping segments of the complete mitochondrial DNA (mtDNA) sequence of each breed. The sizes of the complete mitochondrial genomes of the sHL, AL, and SD breeds were 16,617 bp, 16,613 bp, and 16,613 bp, respectively. The mitochondrial genomes were deposited in the GenBank database with accession numbers KP702285 (AL sheep), KP981378 (SD sheep), and KP981380 (sHL sheep) respectively. The organization of the 3 analyzed sheep mitochondrial genomes was similar, with each consisting of 22 tRNA genes, 2 rRNA genes (12S rRNA and 16S rRNA), 13 protein-coding genes, and 1 control region (D-loop). The NADH dehydrogenase subunit 6 (ND6) and 8 tRNA genes were encoded on the light strand, whereas the rest of the mitochondrial genes were encoded on the heavy strand. The nucleotide skewness of the coding strands of the 3 analyzed mitogenomes was biased toward A and T. We constructed a phylogenetic tree using the complete mitogenomes of each type of sheep to allow us to understand the genetic relationships between Chinese breeds of O. aries and those developed and utilized in other countries. Our findings provide important information regarding the O. aries mitogenome and the evolutionary history of O. aries inside and outside China. In addition, our results provide a foundation for further exploration of the taxonomic status of O. aries.