• 디지털산업정보학회논문지
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• 제12권4호
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• pp.1-12
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• 2016

Digital imaging technology has developed into a state-of-the-art IT convergence, composite industry beyond the limits of the multimedia industry, especially in the field of smart object recognition, face - Application developed various techniques have been actively studied in conjunction with the phone. Recently, face recognition technology through the object recognition technology and evolved into intelligent video detection recognition technology, image recognition technology object detection recognition process applies to skills through is applied to the IP camera, the image object recognition technology with face recognition and active research have. In this paper, we first propose the necessary technical elements of the human factor technology trends and look at the human object recognition based spFACS (Smile Progress Facial Action Coding System) for detecting smiles study plan of the image recognition technology recognizes objects. Study scheme 1). ASM algorithm. By suggesting ways to effectively evaluate psychological research skills through the image object 2). By applying the result via the face recognition object to the tooth area it is detected in accordance with the recognized facial expression recognition of a person demonstrated the effect of extracting the feature points.

• BMB Reports
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• 제37권3호
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• pp.314-319
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• 2004

Flounder (Paralichthys olivaceus) Immunoglobulins (Igs) were purified from the serum of mouse IgG-immunized flounder by using affinity chromatography. Under denaturing conditions in SDS-PAGE, the flounder Igs appeared to be composed of 2 heavy (H) chains (72 and 77 kDa) and two light (L) chains (26 and 28 kDa). Monoclonal antibodies (MAbs) were produced by the fusion of myeloma cells (SP2/0) with Balb/c mouse spleen cells that were previously sensitized against affinity-purified flounder Igs. In a Western blot analysis, the produced MAbs, FIM511, FIM519, and FIM562 recognized both the 72 and 77 kDa H chains, 26 kDa, and 28 kDa L chain, respectively. Mouse antiserum against flounder Igs reacted more strongly with the L chain of 28 kDa than with 26 kDa, suggesting that the 28 kDa molecule is more immunogenic than the 26 kDa L chain molecule. In a FACS analysis, the ratios of the Ig+ cell population in the flounder head kidney and spleen cells were 49% and 24%, respectively. Unexpectedly, however, the ratios of the Ig+ B-like cell population in the flounder were not significantly augmented, even after the immunization of an immunogenic antigen. This suggests that the humoral immune response in fish could be considerably different from that in mammals. The produced MAbs in this study would be useful in characterizing flounder Ig+ B-like cells and in developing flounder Ig detecting an immunoassay system.

• Asian-Australasian Journal of Animal Sciences
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• 제14권8호
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• pp.1179-1187
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• 2001

In fish both humoral and cell mediated immune responses have been reported whereas antibodies recognizing specific cellular populations have not yet been developed except for ones recognizing surface Ig molecules on B lymphocytes. Our aim was to develop and characterize monoclonal antibodies (Mabs) specific for the immune-related cells. Mabs were produced by fusion of myeloma cells (SP2/0) with Balb/c mouse spleen cells previously sensitized against Israeli carp (I. carp) kidney mononuclear cells. We obtained 44 Mabs positively reacting with I. carp kidney mononuclear cells and partially characterized 7 Mabs in the morphological and mitogen-based proliferative aspects. Fluorescence-activated cell sorter (FACS) analysis against I. carp kidney cells by using 7 different Mabs showed 80.3% for ICK 17-4, 65.1% for ICK 2-3, 64.1% for ICK 25-1, 67.5% for lCK 22-1, 70.8% for ICK 16-2, 76.8% for ICK 13-2, 79.7% for ICK II-I. Panning method was used for the isolation of Mabs specific mononuclear carp spleen cells followed by Wright's stain. The stained cell populations were identified as monocytes (ICK 17-4, ICK 2-3, ICK 25-1, ICK 22-1 and ICK 16-2), lymphocytes (ICK 11-1), and a mixed cell population of monocytes and lymphocytes (ICK 13-2). In cell proliferation assay, monocytes purified by ICK 17-4, 2-3 and 22-1 efficiently responded to Con A and PHA, while ones separated by ICK 25-1 did not react with any mitogens. Lymphocytes isolated by ICK 11-1, though it is not known whether they are T or B cells, were more responsive to Con A than PHA or LPS, suggesting that fish immune cells are somewhat different from mammalian cells in responding to mammalian T or B cell mitogens.

• 대한바이러스학회지
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• 제29권2호
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• pp.129-136
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• 1999

Transient transfection assay has been done to evaluate whether the c-jun activation would be prerequisite to the induction of permissiveness against human cytomegalovirus using in vitro cell model in which U937 has been induced to express CD11b and CD14 to become potential monocyte/macrophage cells by TPA treatment. U937 cells were treated with $10\;{\mu}M$, $50\;{\mu}M$ or $100\;{\mu}M$ of TPA. The cell morphology change was observed and the expression of the CD11b and CD14 was confirmed by FACS. Differentiated cells were transfected with pJLuc reporter vector which contained the wild type murine c-jun promoter spanning the SP1, CTF, ATF/CREB and MEF-2 binding sites upstream of the firefly luciferase gene. After 48 hrs of transfection, the cells were infected with HCMV Towne strain and the luciferase activity was assessed at 1 hand 4 h pi. The transfection assay showed no activation of the c-jun promoter at 1 h pi, instead, it showed 2 times increase of the its activity at 4 h pi. There was no difference of the c-jun promoter activation between TPA treated and untreated U937 cells, implying that c-jun activation might not be prerequisite for allowing cells to be premissive to HCMV, although HCMV infection itself could activate c-jun promoter.

• Animal cells and systems
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• 제1권1호
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• pp.157-164
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• 1997

Ly-6E.1 antigen was proposed as a regulatory molecule of T lymphocyte activation, a hematopoietic stem cell marker, a memory cell marker, and an adhesion molecule. Though there were several reports suggesting the presence of Ly-6 ligand, the characterization of the ligand was not yet performed, As an attempt to screen the expression of Ly-6E.1 ligand, we prepared a probe for detecting Ly-6E.1 ligand by producing a fusion protein between Ly-6E.1 and $hlgC_{r1}$, A mammalian cell expression vector with Ly-6E.$1/hlgC_{r1}$ chimeric cDNA was transfected in SP2/0-Ag14 myeloma cells, and stable transfectants were selected. The fusion protein was produced as a dimer and maintained the epitopes for monoclonal antibodies specific for Ly-6E.1 and for anti-human lgG antibody. The purified fusion protein through Gammabind G column was used for FACS analyses for the expression of Ly-6E.1 ligand. The fusion protein interacted with several cell lines originating from B cells, T cells, or monocytes. The fusion Protein also strongly stained bone marrow, lymph node, and spleen cells, but thymic cells weakly, if any. The staining was more obvious in C57BL/6 $(Ly-6^b)$ than Balb/c $(Ly-6^a)$ mice. These results suggest that the interaction of Ly-6E.1 with Ly-6E.1 ligand may function both in the stem cell environment and in the activation of mature lymphocytes. The fusion protein may be a valuable tool in characterization of biochemical properties of the Ly-6E.1 ligand and, further, in isolating its cDNA.

• 생명과학회지
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• 제34권7호
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• pp.500-508
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• 2024

최근 현대인들의 다중이용시설 사용 빈도가 증가하면서 실내 공기 질, 특히 실내공기 오염원인 공기매개 전염성 세균 및 바이러스 불안에 대한 관심이 높아져 다양한 형태의 공기청정기와 공기살균기의 보급이 확산되고 있다. 따라서 공기 내 미생물을 살균할 수 있는 기술에 대한 연구 필요성이 대두되고 있다. 본 연구에서는 염촉매 전기분해 공기살균기를 개발하여 공기살균기의 항균활성과 인간 세포주(HaCaT, BEAS-2B, THP-1)에 대한 세포독성을 통한 안전성을 조사하였다. 공기살균기에서 분무되는 증기를 각각 1, 3시간 동안 분무한 결과, Staphylococcus aureus는 각각 24.01, 57.34%, Bacillus subtilis는 10.89, 57.76%, Escherichia coli는 30.79, 36.59%, Pseudomonas aeruginosa는 34.80, 49.51%, Salmonella typhimurium는 39.40, 73.98%, 진균인 Candida albicans는 36.59, 53.05%의 높은 항균활성을 보여 염촉매 전기분해 공기살균기의 살균효능이 모든 종류의 시험균주에서 시간 의존적인 항균활성을 보였다. 공기살균기의 분무액을 0.1, 0.3, 1.0%의 농도로 처리하고 세포 생존율을 측정한 결과, 1.0%의 농도에서도 BEAS-2B 세포는 93.88%, HaCaT 세포는 97.01%, THP-1 세포는 86.56%로 관찰되어 인체 정상 세포주에서는 유의적인 세포독성을 나타내지 않았다. 또한 분무액을 1.0%의 농도로 처리하고 현미경으로 관찰한 세포주의 형태학적 변화, PCR을 이용한 세포사멸관련 유전자(Bcl-2, Bax)의 발현 분석, FACS를 이용한 세포 내 ROS의 생성 변화 등에서 분무액을 처리하지 않은 대조군과 비교하였을 때 유의적인 변화가 없었다. 따라서 시험균주에 대한 항균활성, 3가지의 인간 세포주에 대한 세포독성, 세포의 형태적 변화, 유독한 반응성 산소(ROS) 생성, 세포사멸관련 유전자의 발현 등에서 유의미한 변화가 확인되지 않아 공기살균기의 살균 효능과 사용상 안전성을 확인할 수 있었다. 최종적으로 다중이용시설에서의 공기살균기의 효능을 조사하기 위하여 밀폐된 실내에서 공기살균기를 20시간 동안 가동한 후, 공기 중의 낙하균을 포집하여 배양한 결과, 총세균은 89.4%, 대장균과 진균은 100.0% 제거되는 것을 확인하였다. 결론적으로 개발된 염촉매 전기분해 공기살균기는 인체에 대한 독성이 없으면서 실내 오염원인 미생물들을 효과적으로 제거할 수 있음을 확인하였다.