• BMB Reports
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• 제29권3호
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• pp.205-209
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• 1996

To investigate the role of heparin in keratinocyte growth factor (KGF) and acidic fibroblast growth factor (aFGF) high affinity binding to the KGF receptor (KGFR), a cell free system was established which utilized a secreted chimeric molecule between the KGFR extracellular domain and the immunoglobulin heavy chain Fc domain (KGFR-HFc). KGFR-HFc was purified from NIH 3T3 cells and demonstrated the binding of $[^3H]-heparin$ as well as heparin Sepharose. Scatchard analysis showed that the dissociation constant for heparin binding to KGFR-HFc was 140 nM. High affinity KGF and aFGF binding to KGFR-HFc remained unchanged after treatment with 0.6 M NaCl, which is the concentration sufficient to release any bound heparin to the KGFR-HFc. These results strongly suggest that although the KGFR interacts with heparin, the presence of heparin is not absolutely required for high affinity binding of either KGF or aFGF to the KGFR.

• KSBB Journal
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• 제14권3호
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• pp.273-278
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• 1999

The molecularly imprinted polymers(MIPs) synthesized at various polymerization conditions were examined as ibuprofen receptors in terms of binding characteristics. The 4-vinylpyridine polymers had 1.2 times higher adsorption capability for (S)-(+)-ibuprofen than the methacrylic acid polymers. The methacrylic acid polymers synthesized by UV radiation had 1.9 times higher selectivity for (S)-(+)-ibuprofen compared to those by thermal initiation. Effects of various solvents for binding were also examined in this research. According to the Scatchard analysis, the (S)-(+)-ibuprofen artificial receptors had two different kinds of binding sites for (S)-(+)-ibuprofen while having only single kind of binding site for ketoprofen. The binding sites of (S)-(+)-ibuprofen, n were calculated as 4.3~4.9 $\mu$mol/g and the dissociation constants, $K_D$ were 0.68 mM for the specific binding.

• Bulletin of the Korean Chemical Society
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• 제22권2호
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• pp.145-148
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• 2001

The interaction between tetradecyl trimethyl ammonium bromide (TTAB) with bovine ${\alpha}-lactalbumin$ has been investigated at pH = 9 and at $37^{\circ}C$ by isothermal titration calorimetry, equilibrium dialysis and UV-Vis spectrophotometry methods. The binding data from unusual Scatchard plot have been analyzed in terms of the Hill equation for three sets of binding sites. The calorimetric data show that TTAB interacts endothermically with ${\alpha}-lactalbumin$ and causes protein unfolding below 2 mM concentration of TTAB, which is confirmed by spectrophotometric data. The unfolding of the protein would be mainly due to occupation of the second set of binding sites.

• 대한핵의학회지
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• 제29권1호
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• pp.98-104
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• 1995

필자는 서울대학교 의과대학 병리학 교실에서 만든 항 백혈병 항체(항 CALLA 항체, 항 JL-1 항체)에 대해 $^{99m}Tc$과 $^{125}I$의 표지 방법 및 면역학적 성상을 연구하여 임상 응용의 토대를 만들고자 하였다. $^{99m}Tc$은 pretargeting transchelation법으로 $^{125}I$는 lodogen법으로 표지하였다. 각 항체에 대해 결합 반응검사, Scatchard 분석, 변조 현상 검사를 시행하였다. $^{125}I$는 두 항체 모두에서 90%전후의 높은 표지율을 보인 반면, $^{99m}Tc$ 경우 70%이하의 표지율을 보여 개선점이 요구되었다. 결합반응검사에서도 $^{99m}Tc$을 표지한 항체는 30%정도의 낮은 면역 반응성을 보였다. Scatchard 분석 결과 결합상수 모두가 $10^9$으로 좋은 친화력을 보였고, 세포당 항체 결합 수는 $10^4$으로 비교적 높은 농도로 나타났다. 변조 현상은 모든 경우에서 나타나지 않았다. 항 CALLA 항체, 항 JL-1 항체는 향후 림프종과 백혈병의 진단 및 치료에 도움이 될 수 있으리라 기대된다.

• KSBB Journal
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• 제18권2호
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• pp.100-106
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• 2003

의학, 약학적으로 작용이 뛰어난 약리성분이 인체 내에서 상처 부위에 얼마나 빨리 도달하여 치료를 하는지를 알기 위하여 혈장 단백질과 약리성분의 결합력을 연구하는 새로운 연구 분야가 HPFA이다. 본 연구는 인체 내에 존재하는 혈장단백질과 항암제로서 알려져 있는 (S)-perillyl alcohol의 결합력과 결합 매개변수를 구하기 위하여 on-line frontal analysis HPLC system을 적용하였다. Develosil 100 Diol 5 (10 cm $\times$ 4.6 mm I.D.)의 HPFA 컬럼을 이용하였고, 이동상은 인산완충용액(pH = 7.4, I = 0.17)을 이용하였다. UV wavelength 205 nm에서 실험을 수행하였고, 주입 부피는 본 실험 조건인 혈장 단백질이 350 rM일 경우에 최대의 혈장 단백질과 결합되지 않은 약리성분의 농도를 갖게 되는 600 ${\mu}\ell$으로 정하였다. Scatchard analysis를 통한 연구 결과로 혈장 단백질인 HSA와 (S)-perillyl alcohol의 결합 매개변수(K)와 단위 HSA에 대한 S-POH의 결합 위치의 수(n)는 각각 K : 2.05 $\times$ $10^{6}$ [M$^{-1}$], n : 0.00428로 실험적으로 구하였다

• 한국작물학회지
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• 제36권6호
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• pp.506-512
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• 1991

IAA에 대한 단크론 항체를 생산하고 이를 이용하여 생체중의 내생 IAA를 정량분석하기 위해 ELISA를 개발하고 본법을 사용하여 담배 종자 발아중 내생 IAA함량을 정량분석하였다. 그 결과는 1. IAA에 대한 단크론 항체 생산 세포주 3가지를 선발 작성하였으며 이 세포주로부터 생산되는 항체는 모두 IgG$_1$ 타입의 면역 글로블린이었다. 2. 상기 항체를 사용하여 ELISA를 수행하여 표준곡선을 작성하였던 바 검출 한계는 1pmol이었으며 검출 범위는 500pmol이었다 3. 표준곡선으로부터 작성한 Scatchard plot에 의한 친화 상수와 결합상수는 6.7$\times$$10^{-10}$ L/M과 6$\times$$10^{-10}$ L/M이었다. 4. 여러가지 IAA유사물질과 교차반응에 의해서 본 mAb는 특이성이 매우 높고 RIA에 의해서 고역가임을 확인하였다 5. 발아중인 담배종자로부터 면역측정에 의해서 내생 IAA를 정량분석하였다 6. 상기의 결과에 따라서 본 mAb를 이용하여 생체중의 내생 IAA를 간편하게 정밀 분석할 수 있음을 확인하였다.

• 약학회지
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• 제32권2호
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• pp.101-111
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• 1988

$[^3H]$ Quinuclidinyl benzilate(QNB) binding assays were performed in the dog ventricular sarcolemma fraction enriched approx. 32-fold in sarcolemma compared to the starting homogenate to elucidate the effect of antihistaminics on cardiac muscarinic receptor. Chlorpheniramine(CHP) inhibited specific binding of $[^3H]$QNB and delayed the equilibrium binding. The rate constants at $37^{\circ}C$ for formation and dissociation of the QNB receptor complex were $0.38{\times}10^9\;M^{-1}$ and $1.6{\times}10^{-2}\;min^{-1}$, respectively. The mean value for the dissociation constant from the pairs of the rate constants was 43. 2 pM and this value was similar to the value(44.8pM) determined from Scatchard analysis. CHP decreased association rate constant, indicating increase in $K_D$ value. Decrease in affinity without affecting the binding site concentration$(B_{max})$ for $[^3H]$QNB binding by CHP was also demonstrated by Scatchard analysis. $K_i$ values for $H_i$-blockers that inhibited specific $[^3H]$QNB binding were $0.02{\sim}4.8{\mu}M$. Cimetidine with $K_i$ value of $230{\mu}M$, however, was ineffective in displacing $[^3H]$QNB binding at concentration of $50{\mu}M$. The Hill coefficient for $H_1$-blockers were about one. The results indicate that $H_1$-antihistaminics inhibit $[^3H]$ QNB binding by interaction with myocardiac muscarinic cholinergic receptor and anticholinergic side effects of these drugs are mainly due to this receptor blocking mechanism.

• Bulletin of the Korean Chemical Society
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• 제25권6호
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• pp.791-795
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• 2004

The binding of cethyl trimethylammonium bromide, (CTAB) with human serum albumin (HSA) has been investigated at 5 mM phosphate buffer pH 7.0, 27 $^{\circ}C$ and various ionic strength using ion selective membrane electrodes. This method is faster and much more accurate than equilibrium dialysis technique, so provides sufficient and accurate data for binding data analysis. A novel and simple method was introduced for resolution and characterization of binding sets on basis of binding capacity concept. The values of Hill binding parameters were estimated for each set and used for calculation of intrinsic binding affinity. The results interpreted on basis of nature of forces which interfered in the interaction and represent the existence of three and two binding sets for binding of CTAB at $10^{-4}$ and $10^{-3}$ M of NaBr, respectively.

• Tuberculosis and Respiratory Diseases
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• 제42권6호
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• pp.801-812
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• 1995

CR asthma is associated with disease chronicity, a positive family history of asthma and in vitro and in vivo defects in mononuclear cell function. The HPA axis in CR asthmatics is suppressed normally by dexamethasone and the pharmacokinetic profile of an oral dose of prednisolone is similar to that found in CS subjects. In addition, competitive binding studies have shown that the ligand binding and nuclear translocation functions of the GR are similar in the two groups. Studies using gel retardation assay have indicated a defect in DNA binding in CR subjects. Chemical mutational analysis of the GR has shown that is not due to a defect in its structure at the cDNA level. Scatchard analysis of the GR/DNA and GR/ligand interactions suggests that there may be transcriptional interference of the GR with other transcriptionally active molecules leading to defective gene transcription.

• Bulletin of the Korean Chemical Society
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• 제34권6호
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• pp.1839-1844
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• 2013

Molecularly imprinted microsphere for chloramphenicol (CAP) with high adsorption capacity and excellent selectivity is prepared by aqueous suspension polymerization, in which chloramphenicol is used as template molecule and ethyl acetate as porogen. The CAP-imprinted microspheres are used as high performance liquid chromatography (HPLC) stationary phase and packed into stainless steel column ($150mm{\times}4.6mm$ i.d.) for selective separation of chloramphenicol. HPLC analysis suggests that chloramphenicol can be distinguished from not only its structural analogs but also other broad-spectrum antibiotic such as erythromycin and tetracycline. In addition, the binding experiments of CAP-imprinted microspheres are carried out in ethanol/water (1:4, V:V), the results indicate that the maximum apparent static binding capacity of molecularly imprinted microspheres is up to 66.64 mg $g^{-1}$ according to scatchard model.