• Journal of Plant Biotechnology
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• 제1권1호
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• pp.13-19
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• 1999

The visco-elastic properties of gluten are major determinants of the processing properties of doughs. These visco-elastic properties are strongly influenced by the ratio of monomeric and polymeric proteins and the size distribution of the polymeric proteins, which make up the gluten fraction of the dough. Recent studies have revealed that other features, such as the number of the cysteine residues of the HMW-GS, also play an important role in determining the functional characteristics. To modify the processing properties at molecular level, the relationship between the structure of molecules and dough properties has to be understood. In order to explore the relationships between individual proteins and dough properties, we have developed procedures for incorporating bacterially expressed proteins into doughs, and measuring their functional properties in small-scale equipment. A major problem in investigating the structure/function relationships of individual seed storage proteins is to obtain sufficient amounts of pure polypeptides from the complex families of proteins expressed in the endosperm. Therefore, we have established a simplified model system in which we produce specific protein genes through bacterial expression and test their functional properties in smallscale apparatus after incorporation into base flour. An S poor protein gene has been chosen as a template gene. This template gene has been modified using standard recombinant DNA techniques in order to test the effects of varying the number and position of cysteine residues, and the size of the protein. Doughs have been mixed in small scale apparatus and characterized with respect to their polymeric composition and their functional properties, including dough mixing, extensibility and small scale bating. We conclude that dough characteristics can be manipulated in a predictable manner by altering the cysteine residues and the size of high molecular weight glutenins.

• 한국작물학회지
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• 제30권2호
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• pp.195-200
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• 1985

유전자 재조합 기술을 통하여 유용한 유전자를 세포내로 이전시키거나 세포 수준에서 육종선발을 하기 위한 기술로서 원형질체를 나출, 배양하고 재분화시키는 과정과 세포주를 확보하기 위하여 실험한 결과를 요약하면 다음과 같다. 1. 원형질체 나출을 위한 잎의 표면 소독은 sodium hypochloride 2 %에서 3분간 침지하는 것이 소독율이 높았다. 2. 원형질체 나출 최적 효소농도는 cellulase 2 %와 macerozyme 0.5 %의 혼용이다. 3. 원형질체의 배양밀도는 1.4 - 2.0 $\times$ $10^4$/$m\ell$에서 치상효율이 높았다. 4. 배양배지는 배지 1에서 제일 양호하였다. 5. 배양 2 일 후에는 세포격이 완전히 재생되고 배양 4 일 후에는 세포분열이 시작되었다. 배양 2주 후에는 세포 덩어리를 형성하고 3주 후에는 육안으로 볼 수 있는 colony를 형성하였다. 6. Shoot 분화 배지에 치상한 calli는 치상후 25 일에 bud가 나타나기 시작하였다. Shoot분화에는 BA 1 -2 mg/$\ell$로 첨가한 경우 shoot분화율이 높았다. 7. 발근은 홀몬이 첨가되지 않은 MS 배지에서 양호하였고 현재 100여 개의 세포주에서 종자를 수확하였으며 차후 세포주의 특성과 변이성등을 조사할 계획이다.

• 대한수의학회지
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• 제25권1호
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• pp.7-17
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• 1985

Many investigators have been pursuing various attempts so far to produce hepatitis B surface antigen(HBsAg) vaccines using the techniques such as isolation from plasma of chronic HBsAg carrier, recombinant DNA technique or preparation of synthetic peptides specific for immunogenic determinants. Hepatitis B virus can not grow on any cell lines by the tissue culture technique at the present time. The plasma of chronic HBsAg carrier is expensive and its source is limited. The HBsAg from the recombinant DNA technique gave still very low yield. Another approach, therefore, has been initiated to develop a synthetic hepatitis B virus vaccine. The possible use of several distinct synthetic vaccines in prophylaxis can be facilitated by availability of full synthetic immunogens. Peptides synthesized for potential application as antiviral vaccines have been mostly tested in the form of conjugates with carrier proteins, although the free synthetic peptide can be immunogenic. To understand basic knowledges on the antigenicity and immunogenicity of a synthetic peptide specific for major immunogenic determinant of HBsAg, a nonapeptide, $H_2N^{139}Cys-Thr-Lys-Pro-Thr-Asp-Gly-^{146}Asn-Aba$ COOH, which corresponds to HBsAg amino acid residues 139 to 147, was synthesized by the Merrifield's solid-phase method with a slight modification. The antigenicity and immunogenicity of this specific synthetic peptide were examined comparing with purified plasma-derived natural HBsAg. The results obtained are as follows; 1. The peptide synthesized showed the identical amino acid composition to the theoretical value. The degree of purification and molecular weight were acertained by methods of high performance liquid chromatography and mass spectrometry. 2. Using m-maleimidobenzoyl-N-hydroxysuccinimide ester as a conjugating agent, the synthetic peptide was conjugated to rabbit albumin and ${\gamma}$-globulin, tetanus and diphtheria toxoids, and keyhole limpet hemocyanin. Their conjugation yields were 8.3, 9.5, 15.8, 13.5, and 11.2%, respectively. 3. The natural HBsAg was purified from plasma of chronic HBsAg carrier. By the electron microscopic observation of the purified natural HBsAg preparation, no Dane particles were observed and the preparation showed negative DNA polymerase activity. 4. Antigenicity of the synthetic peptide and the plasma-derived natural HBsAg was determined by competition radioimmunoassay using $^{125}I$-natural HBsAg. Their 50% inhibitions appeared as $90{\mu}g/ml$ and $0.12{\mu}g/ml$ for the synthetic peptide and the natural HBsAg, respectively. This indicates that the former was about 750-fold less antigenic than the latter. 5. Immunogenicity of the synthetic peptide was determined by administering the peptide-carrier conjugates into rabbits with and without Freund's complete adjuvant. Regardless the carrier proteins and adjuvant, positive immune responses to the synthetic peptide were observed. The higher antibody titers, however, were shown in the groups administered with Freund's complete adjuvant. 6. Immunizing dose 50% in mice of the various peptide-carrier conjugates was 5.47, 6.00, 65.16, 31.25 and $13.03{\mu}g/dose$ for rabbit albumin and ${\gamma}$-globulin, tetanus and diphtheria toxoids, and keyhole limpet hemocyanin, respectively, while the natural HBsAg showed $0.65{\mu}g/dose$. 7. It was postulated that homologous proteins prefer to heterologous ones as the carriers.

• 미생물학회지
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• 제27권3호
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• pp.176-180
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• 1989

E. coli의 $tRNA^{phe}$내에는 세 개의 psiudouridine 염기들이 존재한다. 이 $tRNA^{phe}$내의 pseudouridine 염기들의 기능을 연구하기 위하여 부위특이적 돌연변이를 이용하여 $tRNA^{phe}$ 유전자의 염기를 다른 염기로 치환시켰다. E. coli $tRNA^{phe}$ 유전자들 중 하나인 phe W 유전자내에서 32번에 해당하는 T 염기를 C 염기로 39번 T 염기를 C 염기로 Kunkel이 개발한 부위특이적 돌연변이 방법을 사용하여 각각 치환시켰다. DNA 염기서열을 결정함으로써 돌연변이체를 확인하였으며, 이들 돌연변이 유전자를 함유한 재조합 플라스미드를 이용하여 돌연변이된 phe W 유전자들의 E. Coli NP37($pheS^{-ts}$)에 대한 complementation 활성을 조사하였다. 32번 위치가 변이된 pheW 유전자 뿐만아니라 39번 위치가 변이된 phe W 유전자를 함유한 E. coh NP37들은 모두 non-permissive temperature에서 자라지 못하였다. 이 결과는 변이된 pheW 유전자들이 E. coli NP37을 complementation 할 수 없으며, 또 pseudouridine 염기들이 생체내에서 E. coli $tRNA^{phe}$의 활성에 필수적이라는 것을 의미한다.