• The Korean Journal of Physiology
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• 제30권2호
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• pp.209-218
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• 1996

Acetylcholine (ACh) activates the inwardly rectifying muscarinic $K^{+}$ channel in rat atrial cells via pertussis toxin (PTX)-sensitive G-protein ($G_k$) coupled with the muscarinic receptor (mAChR). Although this $K^{+}\;(K_{ACh})$ channel function has reported to be modulated by the phosphorylation process, a kinase and phosphatase involved in these processes are still unclear. Since either PKA or PKC was not effective on this ATP-modulation, the present study examined the possible involvement of the protein tyrosine kinase (PTK) and protein tyrosine phosphatase (PTP) in the function of the $K_{ACh}$ Channel. In the inside-out (I/O) patch preparation excised from the adult rat atrial cell, when activated by 10 ${\mu}M$ ACh in the pipette and 100 ${\mu}M$ GTP in the bath, the mean open time (${\tau}_{o}$) and the channel activity ($K_{ACh}$) was 1.13 ms (n=5) and 0.19 (n=6), respectively. Following the application of 1 mM ATP into the bath, ${\tau}_{o}$ increased by 34% (1.54 ms, n=5) and $K_{ACh}$ by 66% (0.28, n=6). Channel function elevated by ATP was lasted after washout of ATP. However, this ATP-induced increase in the $K_{ACh}$ channel function did not occur in pretreated cells with genistein ($50{\sim}100 {\mu}M$), a selective PTK inhibitor, but occurred in pretreated cells with equimolar daidzein, a negative control of the genistein. On the contrary, PTP which acts on tyrosine residue conversely reversed both ATP-induced increased ${\tau}_{o}$ by 32% (1.20 ms, n=3) and $K_{ACh}$ by 41% (0.15, n=3), respectively. Taken together, these results suggest that $K_{ACh}$ channel may, at least partly, be regulated by the tyrosyl phosphorylation, although it is unclear where this process exerts on the muscarinic signal transduction pathway comprising the mAChR-$G_{k}$-the $K_{ACh}$ channel.

• The Korean Journal of Physiology
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• 제28권2호
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• pp.133-141
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• 1994

The discharge patterns and peripheral nerve inputs to cardiovascular neurons were investigated in rostral ventrolateral medulla (RVLM) and raphe nucleus of cats. The data from the two were compared to determine their roles in cardiovascular regulation and the endogenous analgesic system. Animals were anesthetized with ${\alpha}-chloralose$ and single cell activities were recorded by carbon-filament microelectrode and their relationships with cardiovascular activity were analyzed. In RVLM area, a total of thirty-three cells were identified as cardiovascular neurons. During one cardiac cycle, the mean discharge rate of the neurons was $1.96{\pm}0.29$ and the peak activity was observed 45 ms after the systolic peak of arterial blood pressure. Thirteen cells could be activated antidromically by stimulation of the the $T_2$ intermediolateral nucleus. Forty-three raphe neurons were identified as cardiovascular neurons whose mean discharge rate during one cardiac cycle was $1.02{\pm}0.12$. None of these cells could be activated antidromically. Study of the interval time histogram of RVLM neurons revealed that the time to the first peak was $128{\pm}20.0\;ms$, being shorter than the period of a cardiac cycle. The same parameter found from the raphe neurons was $481{\pm}67.2\;ms$, which was much longer than the cardiac cycle length. Of seventeen RVLM neurons examined ten received only the peripheral $A{\delta}-afferent$ inputs, whereas six RVLM neurons received both $A{\delta}-$ and C-inputs; the remaining one cell received an inhibitory peripheral C-input. In contrast, nine of eleven raphe neurons were found to receive $A{\delta}-inputs$ only. We conclude that the main output of cardiovascular regulatory influences are mediated through the RVLM neurons. The cardiovascular neurons in the raphe nucleus appear to serve as interneurons transferring cardiovascular afferent information to the raphespinal neurons mediating the endogenous analgesic mechanisms.

• The Korean Journal of Physiology
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• 제23권2호
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• pp.313-328
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• 1989

The electrophysiological properties of the inward current contributing to the late plateau phase of the action potential were investigated using the whole cell clamp technique and intracellular dialysis in single atrial cells isolated from the rabbit heart. The inward current was activated by various repolarizing pulses after a brief depolarizing pulse to +40 mV for 2 ms and its time course was similar to that of the late plateau of the action potential. The current was fully activated above the potential of -40 mV and abolished by intracellular EGTA. Ryanodine of $1{\mu}M$ also abolished the late plateau and the inward current. Reduced $Na_o\;to\;30%\;and\;20\;mM\;Na_1$ diminished the late plateau together with the inward current. Diltiazem blocked the activation of the current and Ni in the concentration of $40{\sim}200\;{\mu}M$ decreased the development of the late plateau and the inward current. Fully activated current-voltage relation of the inward current showed exponential voltage dependency which was steeper in more hyperplarizing range. The above findings suggest that the inward current was activated by intracellular calcium and contribute the late plateau phase of the action potential. It could be concluded that the inward current would be the inward component of Na-Ca exchange.

• 한국가정과학회지
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• 제4권1호
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• pp.79-92
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• 2001

본 연구에서는 미생물의 대사체계를 이용하여 유자껍질내의 유자정유성분을 생전환 시키므로써 고부가가치 고기능성 천연향의 발굴 생산을 시도하였다. 유자정유 성분 대사능 유전자를 지닌 E. coli 형질전환주 EC3, EC4, EC6의 공동 배양액을 유자정유가 유일한 탄소원인 M9배지에서 28$^{\circ}C$로 진탕배양 하였다. 각 공동 배양액(EC3+EC4. EC3+EC6, EC4+EC6 and EC3+C4+EC6)은 각 형질전환주의 단독배양 보다 3∼4배 더 높은 생육도를 나타냄을 알 수 있었다. 공동배양에 의해 생전환된 물질들은 GC-MS에 의해 확인하였다. 각 공동배양액의 주요한 대사산물로는 linalool, 4-terpineol, ${\alpha}$-terpineol이 공통적으로 검출되었다. 소량씩 존재하나 배양액의 주요한 향을 결정할 것으로 보이는 각기 다른 terpene 계열 화합물들이 각각의 공동배양액 대사산물로 검출 되었는데, 공동배양액EC3+EC4에서는 elemol, ocimene, nonanal, trans-2-nonenal이 공동배양액EC3+EC6에서는 cis-ocimene, 2-octanol, octanal. ${\alpha}$-terpinolene, 공동배양액 C4+EC6에서는 ocimene, 그리고 공동배양액EC3+EC4+EC6에서는 nonanal, 2-octenol, iso-menthol, ocimene이 각각 검출되었다.

• 한국자원식물학회지
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• 제24권2호
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• pp.121-129
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• 2011

분자육종의 발전에 따라 좀 더 유용한 형질전환 식물체를 더 많이 얻어내기 위한 많은 형질전환 기술들이 개발되어오고 있으나 새로운 수요를 충족시키기 위한 다양한 종류의 새로운 품종들이 실시간으로 새롭게 개발되고 있으며 개발된 품종에 적합한 새로운 형질전환 기술에 대한 개발 필요성 또한 지속적으로 요구되고 있다. 카네이션(Dianthus caryophyllus L.)은 전 세계적인 주요 화훼작물 중 하나로 경제적 파급효과가 매우 큰 작물이다. 따라서 기술개발의 파급효과가 큰 카네이션을 대상으로 조직배양 및 형질전환의 효율성을 향상시키기 위하여 시장에서 주요하게 거래되고 있는 주요 품종 18종을 수집하고 이 중 조직배양을 통한 신초 분화 능력이 우수한 4개 품종 Yellow dotcom, Jakarta, Belmonte, Polar tessino 등을 선발하였다. 선발된 4개 품종에 공통으로 적용시킬 수 있는 가장 효율적인 생장조절제는 MS+Sucrose 3%+NAA 1.0 mg/L+TDZ 1.0 mg/L.이었으며 MS+Sucrose 3%+NAA 3.0 mg/L+BA 1.0 mg/L 처리는 Belmonte.에 적용 가능한 생장조절제 조합이었다. 캘러스 형성과 신초 분화에 가장 효율적인 기본 배지는 MS이었으며 탄소원으로는 Sucrose를 3%로, Phytagel 0.3%를 배지 경화제로 처리하는 것이 조직배양을 통한 재분화 식물체 획득에 가장 효과적이었다. 가장 효율적 조직배양 체계를 구축하기 위한 조직배양 부위는 줄기 부위 이었으며 이 부위를 배양재료로 사용할 경우 신초 생성율을 80.2%까지 올릴 수 있었고 배양소요 기간도 6일 정도 단축할 수 있었다.

• IMMUNE NETWORK
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• 제22권5호
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• pp.40.1-40.24
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• 2022

Mesenchymal stem cells (MSCs) are attractive alternatives to conventional anti-asthmatic drugs for severe asthma. Mechanisms underlying the anti-asthmatic effects of MSCs have not yet been elucidated. This study evaluated the anti-asthmatic effects of intravenously administered MSCs, focusing on macrophages and monocytes. Seven-week-old transgenic (Tg) mice with lung-specific overexpression of IL-13 were used to simulate chronic asthma. MSCs were intravenously administered four days before sampling. We examined changes in immune cell subpopulations, gene expression, and histological phenotypes. IL-13 Tg mice exhibited diverse features of chronic asthma, including severe type 2 inflammation, airway fibrosis, and mucus metaplasia. Intravenous administration of MSCs attenuated these asthmatic features just four days after a single treatment. MSC treatment significantly reduced SiglecF^-CD11c^-CD11b⁺ monocyte-derived macrophages (MoMs) and inhibited the polarization of MoMs into M2 macrophages, especially M2a and M2c. Furthermore, MSCs downregulated the excessive accumulation of Ly6c^- monocytes in the lungs. While an intravenous adoptive transfer of Ly6c^- monocytes promoted the infiltration of MoM and Th2 inflammation, that of MSC-exposed Ly6c^- monocytes did not. Ex vivo Ly6c^- MoMs upregulated M2-related genes, which were reduced by MSC treatment. Molecules secreted by Ly6c^- MoMs from IL-13 Tg mice lungs upregulated the expression of fibrosis-related genes in fibroblasts, which were also suppressed by MSC treatment. In conclusion, intravenously administered MSCs attenuate asthma phenotypes of chronic asthma by modulating macrophages. Identifying M2 macrophage subtypes revealed that exposure to MSCs transforms the phenotype and function of macrophages. We suggest that Ly6c^- monocytes could be a therapeutic target for asthma management.

• 한국진공학회:학술대회논문집
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• 한국진공학회 2016년도 제50회 동계 정기학술대회 초록집
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• pp.340-340
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• 2016

We have prepared alumina (Al2O3) doped zinc oxide (AZO) films by DC magnetron sputtering (MS) technique and obtained higher self surface texturing at a high target angle (f). We have characterized the films and applied it as a front electrode of a single junction amorphous silicon solar cell. At a lower f the deposited films show higher values of optical gap (Eg), charge carriers mobility & concentration, crystallite grain size and wider wavelength range of transmission. At higher target angle the sheet resistance, surface roughness, haze factor etc for the films increase. For f=72.5o the haze factor for diffused transmission becomes 6.46% at 540 nm wavelength. At f=72.5o the material shows a reduction in crystallinity and evolution of a hemispherical-type sub-micron surface textures. A Monte Carlo method (MCM) of simulation of the AZO film deposition shows that such an enhanced self-surface texturing of the films at higher f is possible.

• 한국진공학회:학술대회논문집
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• 한국진공학회 2015년도 제49회 하계 정기학술대회 초록집
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• pp.230.1-230.1
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• 2015

One of the major problems of biological ToF-SIMS imaging is the lack of protein and peptide imaging. Most of biological story telling is mianly based on proteins. The biological implication of lipid ToF-SIMS imaging would be much higher if protein imaging is provided together. Utilizing high secondary ion yields of metals, proteins can be ToF-SIMS imaged with nanoparticle tagged proteins. Nanoparticles such as Fe3O4, SiO2, PbS were used for imaing NeuN, MCH, Orexin A, ${\alpha}$ synucline, TH(Tryosine Hydroxylase) in mouse tissues with a spatial resolution of ${\sim}2{\mu}m$ using a TOF-SIMS. Lipids and neurotransmitters images obtained simultaneously with protein images were overlayed for more deeper understanding of neurobiology, which is not allowed by any other bioimaging technqiues. The protein images from TOF-SIMS were compared with confocal fluorescence microscopy and NanoSIMS images. A new sample preparation method for imaging single cell membranes in a tissue using the vibrotome technique to prepare a tissue slice without any fixation and freeze drying will be also presented briefly for Hippocampus and Hypothalamus tissues.

• KSII Transactions on Internet and Information Systems (TIIS)
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• 제9권8호
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• pp.3054-3067
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• 2015

The phenomena of higher channel cross polarization discrimination (XPD) is mainly observed for future wireless technologies such as small cell network and massive multiple-input multiple-output (MIMO) system. Therefore, utilization of high XPD is very important and space-polarization division multiple access (SPDMA) with dual-polarized MIMO system could be a suitable solution to high-speed transmission in high XPD environment as well as reduction of array size at base station (BS). By SPDMA with dual-polarized MIMO system, two parallel data signals can be transmitted by both vertically and horizontally polarized antennas to serve different mobile stations (MSs) simultaneously compare to conventional space division multiple access (SDMA) with single-polarized MIMO system. This paper analyzes the performance of SPDMA for maximum ratio transmission (MRT) in time division duplexing (TDD) system by proposed dual-polarized MIMO spatial channel model (SCM) compare to conventional SDMA. Simulation results indicate that how SPDMA utilizes the high XPD as the number of MS increases and SPDMA performs very close to conventional SDMA for same number of antenna elements but half size of the array at BS.

• 한국의학물리학회지:의학물리
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• 제21권2호
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• pp.209-217
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• 2010

색소성망막염(retinitis pigmentosa: RP)이나 연령관련 황반변성(age-related macular degeneration: AMD)과 같은 망막질환으로 인해 실명한 환자를 위해 인공시각장치가 개발되고 있다. 인공시각장치의 동작원리는 전기자극을 주어 신경세포의 활동도를 조절하는 것이므로 시각정보를 제대로 인코딩하기 위해 최적의 전기자극을 인가하는 것은 인공시각장치의 실용화를 위해 매우 중요한 요소이다. 그러므로 본 연구에서는 전압자극의 크기와 자극시간을 변화시켜 가면서 정상망막과 변성망막에 인가한 후 자극에 의해 유발된 망막신경절세포 반응을 분석하고 역치전하밀도를 비교함으로써 최적의 전기자극 조건을 찾아보고자 하였다. 이를 위하여 정상마우스와 rd1 마우스의 망막을 in vitro 상태로 분리한 후 망막의 신경절세포층이 전극을 향하여 부착되도록 한 후 망막신호를 기록하였다. rd1 마우스에서 얻은 변성망막의 망막신경절세포에서도 전압펄스를 인가시 정상망막의 망막신경절세포처럼 전압자극의 크기와 자극시간 변조에 대하여 반응하였다. 그러나 정상망막과 변성망막에서 망막신경절세포 반응의 시간적 패턴은 매우 달랐다: 정상망막의 망막신경절세포 반응은 전기자극 후 약 100 ms 내에서 1개의 피크만 나타나는 반면, 변성망막에서는 이보다 긴 400 ms 구간에서 약 10 Hz의 진동리듬을 가진 다수의 피크(~4개)들이 나타나는 것을 확인하였다. 또한 변성망막에서 망막신경절세포의 반응을 유발하기 위한 역치 전하밀도가 정상망막에서 보다 크게 상승하였다: 자극세기를 변화시켰을 때 정상망막의 역치 전하밀도는 $37.23{\sim}61.65\;{\mu}C/cm^2$, rd1 마우스에서는 $70.50{\sim}99.87\;{\mu}C/cm^2$로 2배가량 높은 것을 확인하였다. 자극시간을 변화시켰을 때 정상망막의 역치 전하밀도는 $22.69{\sim}37.57\;{\mu}C/cm^2$, rd1 마우스에서는 $120.5{\sim}170.6\;{\mu}C/cm^2$로 5배가량 높은 것을 확인하였다.