• 생명과학회지
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• 제31권10호
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• pp.944-953
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• 2021

리그닌은 식물의 세포벽에 풍부하게 존재하는 복잡한 phenylpropanoid 중합체이다. 주로 물 수송과 기계적 강도를 유지하는 조직에 존재하며 수분을 운반하거나, 기계적인 지지를 담당한다. 또한, 리그닌은 병원균의 감염이나 상처에 대한 물리적인 장벽으로 작용함으로써 방어 기작에 관여한다. 리그닌을 생성하는 모노리그놀 전구체는 cinnamyl alcohol dehydrogenase (CAD) 유전자에 의해 합성된다. CAD는 cinnamaldehyde를 cinnamyl alcohol(p-coumaryl, coniferyl, sinapyl alcohol)로 전환하는 효소이다. CAD는 속씨식물에서 multigenic family로 존재하며 여러 식물 종에서 다른 기능을 가진 CAD isoform이 밝혀졌다. CAD 유전자의 여러 isoform은 식물의 발달 및 환경 신호에 따라 다르게 발현되었다. 하나의 isoform이 발달 리그닌화에 관여하는 반면, 다른 isoform은 방어 리그닌 및 기타 세포벽에 결합된 페놀의 구성에 영향을 미칠 수 있음을 보여주었다. CAD isoform에 따라 기질 특이성이 다르게 나타나고, 이는 리그닌 합성을 조절하는 CAD 단백질의 생화학적 특성을 나타내는데 기여한다. 본 논문에서는 리그닌 생합성에서 CAD multigenic family 유전자의 발현과 조절에 대하여 설명하였다. CAD multigenic family의 isoform들은 유전적 조절이 복잡하고, 식물 발달 과정의 신호 경로와 스트레스 반응이 밀접하게 연동되어 있다. CAD 유전자에 의한 모노리그놀 합성은 발달 및 환경 신호에 의해 조절될 가능성이 높다.

• Asian-Australasian Journal of Animal Sciences
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• 제12권7호
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• pp.1129-1134
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• 1999

The rapid development of the sheep genetic linkage map over the last five years has given us the ability to follow the inheritance of chromosomal regions. Initially this powerful resource was used to find markers linked to monogenic traits but there is now increasing interest in using the genetic linkage map to define the complex of genes that control multigenic production traits. Of particular interest are those production traits that are difficult to measure and select for using classical quantitative genetic approaches. These include resistance to disease where a disease challenge (necessary for selection) poses too much risk to valuable stud animals and meat and carcass qualities which can be measured only after the animal has been slaughtered. The goal for the new millennium will be to fully characterise the genetic basis of multigenic production traits. The genetic linkage map is a vital tool required to achieve this.

• IMMUNE NETWORK
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• 제10권6호
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• pp.198-205
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• 2010

Background: A crucial limitation of DNA vaccines is its weak immunogenicity, especially in terms of eliciting antibody responses in non-human primates or humans; therefore, it is essential to enhance immune responses to vaccination for the development of successful DNA vaccines for humans. Methods: Here, we approached this issue by evaluating interleukin-7 (IL-7) as a genetic adjuvant in cynomolgus monkeys immunized with multigenic HCV DNA vaccine. Results: Codelivery of human IL-7 (hIL-7)-encoding DNA appeared to increase DNA vaccine-induced antibody responses specific for HCV E2 protein, which plays a critical role in protecting from HCV infection. HCV-specific T cell responses were also significantly enhanced by codelivery of hIL-7 DNA. Interestingly, the augmentation of T cell responses by codelivery of hIL-7 DNA was shown to be due to the enhancement of both the breadth and magnitude of immune responses against dominant and subdominant epitopes. Conclusion: Taken together, these findings suggest that the hIL-7-expressing plasmid serves as a promising vaccine adjuvant capable of eliciting enhanced vaccine-induced antibody and broad T cell responses.

• International Journal of Industrial Entomology and Biomaterials
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• 제11권2호
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• pp.119-124
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• 2005

To determine the level of heterosis, higher cocoon shell weight multivoltine congenic lines (Con. L) and bivoltine syngenic lines (Syn. L) of silkworm were used for crosses. First filial generations $(F_1s)$ expressed heterobeltiotic genetic interaction at significant magnitude (p < 0.01) for single cocoon shell weight (SCSW). The other linked characters viz., single cocoon weight (SCW) and yield by weight per 10, 000 larvae were also significantly higher (p < 0.01) than the better parental lines. All the hybrids showed significant improvement for these aforesaid characters over standard heterosis (Standard check). The reeling parameters viz., filament length, raw silk, neatness, cohesionstrokes etc, also showed improvement among the hybrids than check in congenial environment. Overall results suggested that the cross between congenic and syngenic lines provide better heterosis with good quality silk than conventional hybrids and may be used for commercial exploitation.

• 한국미생물생명공학회:학술대회논문집
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• 한국미생물생명공학회 2004년도 Annual Meeting BioExibition International Symposium
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• pp.236-241
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• 2004

In Escherichia coli, L-lysine biosynthetic pathway is composed of nine enzymatic reactions. It has been well established that most of the lysine biosynthetic genes are regulated by the lysine availability, even though they are all scattered around the chromosome without forming any multigenic operon structure. However, no transcriptional regulatory mechanism has been identified except for the activation of lysA gene by the LysR. In this study, changes in transcriptome profiles of wild type cells and lysR deletion mutant cells grown in the absence or presence of lysine were investigated by using DNA microarray technique. Microarray data analysis revealed three groups of genes whose expression varies depending on the availability of lysine or LysR or both. To further examine the regulatory patterns of lysine biosynthetic genes, lacZ operon fusions were constructed and their expression was measured under various conditions. Obtained results strongly suggest that there is an additional regulatory mechanism which senses the lysine availability and coordinates gene expression.

• Journal of Plant Biotechnology
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• 제40권1호
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• pp.9-17
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• 2013

Ran is a small GTP-binding protein that binds and subsequently hydrolyzes GTP. The functions of Ran in nuclear transport and mitotic progression are well conserved in plants and animals. In animal cells, stress treatments cause Ran relocalization and slowing of nuclear transport, but the role of Ran proteins in plant cells exposed to stress is still unclear. We have therefore compared Ran genes from three EST libraries construed from different cell types of sweetpotato and the distribution pattern of Ran ESTs differed according to cell type. We further characterized two IbRan genes. IbRan1 is a specific EST to the suspension cells and leaf libraries, and IbRan2 is specific EST to the root library. IbRan1 showed 94.6 % identity with IbRan2 at the amino acid level, but the C-terminal region of IbRan1 differed from that of IbRan2. These two genes showed tissue-specific differential regulation in wounded tissues. Chilling stress induced a similar expression pattern in both IbRan genes in the leaves and petioles, but they were differently regulated in the roots. Hydrogen peroxide treatment highly stimulated IbRan2 mRNA expression in the leaves and petioles, but had no significant effect on IbRan1 gene expression. These results showed that the transcription of these two IbRan genes responds differentially to abiotic stresses and that they are subjected to tissue-specific regulation. Plant Ran-type small G-proteins are a multigenic family, and the characterization of each Ran genes under various environmental stresses will contribute toward our understanding of the distinctive function of each plant Ran isoform.

• International Journal of Industrial Entomology and Biomaterials
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• 제8권2호
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• pp.189-194
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• 2004

Amylase isozyme based three multivoltine viz., N+p, Np, N+ $p^{cho}$ and two bivoltine-D6+p, D6p syngenic lines (Syn. L) were developed from germplasm (GP) stocks Nistari (N) and D6 respectively. haemolymph isozyme pattern at pH 7.0 and 8.5 depicted a total 11 number (Am $y_{1 to 6}$ at pH 7.0 and Am $y^{l to 5}$ at pH 8.5) of native proteins (NP) of various sizes are amylase isozyme expressers. Among eleven NPs, two NPs of 770 kDa (Am $y^{6}$ at pH 7.0) and 376 kDa (Am $y^3$ at pH 8.5) are $\alpha$-amylase expressers and remaining NPs of 370, 364, 350, 329 and 274 kDa at pH 7.0 and 206, 292, 416, 725 kDa at pH 8.5 are $\beta$-amylase expressers. Accordingly, digestive juice amylase isozyme pattern at aforesaid pH also depicted a total number of 10 NPs (Am $y^{1 to 5}$) at each pH 7.0 and 8.5 are amylase expressers of which NP of 387 kDa (Am $y^4$ at pH 7.0) and 780 kDa (Am $y^{5}$ at pH 8.5) are a-amylase expresser. Remaining NPs of 338,297 ＆ 216 kDa at pH 7.0 and 370, 341, 329 ＆302 kDa at pH 8.5 are $\beta$-amylase expresser. Recurrent backcross lines (RBL) viz., N+pRBL and NpRBL were developed through introgression of high shell weight character (a multigenic trait) to be used further for congenic line (Con. L) development and to understand any association with introgressed character. Isozyme pattern in haemolymph of RBLs depicted only one $\alpha$-amylase of 770 kDa at pH 7.0 and 376 kDa at pH 8.0 with three and four respective $\beta$-amylase bands but in bivoltine lines numbers of $\beta$-amylase bands vary between 1 to 2 at aforesaid pH. Variability was also observed in digestive juice of multivolitine and its RBLs but bivoltine lines express null activity at both pH except appearance of one very week $\alpha$-amylase band D6+p at pH 8.5. Overall study suggests that not a single NP at both pH is common for expression of any band of amylase isozyme i.e., a totally different set of proteins are the amylase isozyme expresser at specific pH and no molecular factor of amylase is associated in developed RBLs which showed improvement on survival, single cocoon shell weight (SCSW) and single filament length over receptor parents.s.s.s.

• 생명과학회지
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• 제25권12호
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• pp.1458-1469
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• 2015

유기용매 내성 세균의 첫 분리 보고 이후 다수의 유기용매 내성 세균들이 토양 폐수 심지어 심해 등 모든 환경에서 분리 보고되고 있다. 대부분의 유기용매 내성 세균은 그람음성세균으로 이는 그람음성 세균이 그람양성 세균 보다 유전적으로 더 내성을 보이기 때문이다. 유기용매 내성 기전은 유기용매 내성 그람음성 세균을 주로 사용하여 집중적으로 구명되어왔다. 유기용매 내성 그람양성 세균의 유기용매 내성 기전은 비교적 최근 연구에서 발견되고 있다. 유기용매는 용매에 따라 다른 독성을 보이며 유기용매 내성세균의 유기용매 내성 수준은 종과 균주에 의존적으로 매우 변화가 심하다. 그러므로 유기용매 내성세균은 다양한 변인과 다유전자에 의한 적응 전략에 의하여 용매독성과 싸우며 용매 스트레스에 적응할 수 있다. 그들은 세포형태 및 세포 행동에서의 변화, 세포표층의 수식, 세포막 적응, 용매 배출 펌프, 샤페론 그리고 항산화 반응 등의 기전을 통하여 유기용매의 과량의 농도에서도 생존할 수 있다. 본 총설에서는 대표적인 유기용매 내성 세균, 유기용매 내성 세균에서의 유기용매에의 적응 및 내성 전략들 나아가 그들의 산업적 및 환경공학적인 잠재적인 영향에 대하여 개관하고자 한다.