• 보존과학회지
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• 제27권4호
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• pp.345-356
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• 2011

금속산화물에 오염된 도자기 유물을 보존처리 하기 위해서는 경우에 따라 화학적 세척과정이 필요하다. 본 연구에서는 화학적 세척과정을 침적법과 습포법으로 구분하여, 침적법에서는 옥살산과 구연산의 농도에 따른 철산화물 제거특성을 확인하고자 하였다. 나아가 앞선 침적법의 결과를 토대로 spot 테스트를 거친 후, 태안 마도에서 출토된 도자기 유물에 습포법을 적용하여 철산화물을 제거하였다. 옥살산에 60시간 침적시 도자기 빙렬 내의 철산화물은 제거되었지만, 육안관찰에서 침적 3시간 이후부터 철산화물이 관찰되지 않기 때문에 보존처리현장에서는 유물의 안정성을 고려하여 0.25M 이하의 옥살산에 1~3시간동안 침적하는 것이 적당할 것으로 판단된다. 구연산에서는 60시간 침적시 철산화물은 제거되지 않았다. 이는 옥살산과의 분자량 차이 및 산도(acidity) 등에 의한 것으로, 빙렬 내에 침투한 철산화물을 제거할 때에는 구연산보다 옥살산이 좀 더 효과적이었다. 옥살산을 용제로 제작한 습포팩(벤토나이트, 세피올라이트, 활성탄소섬유, 셀라이트)을 오염된 백자태토에 10시간동안 도포 처리하여 철산화물은 제거되었지만, 유물적용성은 벤토나이트와 세피올라이트가 뛰어났다. 그래서 앞선 침적법의 결과를 토대로, 0.25M의 옥살산과 세피올라이트를 습포 팩으로 제조하여 태안 마도 출토 청자 및 백자에 적용하였다. 습포팩 1회 처리로 유물표면의 철산화물은 대부분 제거되었으나 오염물의 형태에 따라 적용횟수는 달라질 수 있을 것으로 판단되며, 세피올라이트에 의한 2차 오염을 방지하기 위한 세척도 함께 병행되어야 할 것이다.

• 대한세포병리학회지
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• 제8권1호
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• pp.27-34
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• 1997

Pneumocystis carinli is an established cause of pulmonary infections in immuno-compromised hosts. Several cytoiogical stains, such as Papanicolaou, Gomori methenamine sliver(GMS) and Diff-Quik have been used for detection of the organism, but occasionally can be laborious and, due to a degree of nonspecificity, may be misleading. We evaluated the diagnostic utility of immunocytochenmical stains that recognize P. carinii in bornchoalveolar lavage from experimentally Induced P. carinii pneumonia rats(n=15). In audition to routine stains for diagnosis by morphologic recognition of P. carinii on Papanicolaou, GMS and Diff-Quik stains, bronchoalveolar lavage samples were reacted with immunocytochemical stains using monoclonal antibodies(MAB) 092 and 902. In bronchoalveolar lavage P. carinii organisms were detected In 9 of 10 cases(90%) using each MAB 092 and 902, whereas GMS and Diff-Quik stains demonstrated P. carinii in 13(86%) and 11(73%) of 15 cases respectively. In lung tissue specimens(n=15) P. carinii organisms were well identified on GMS stain and immunohistochemical stains using MAB 092 and 902 in ail cases. We believe that the immunocytochemical staining using MAB 092 and/or 902 is a very useful and diagnostic tool In addition to GMS and Diff-Qulk stain to detect P. carinii organisms in bronchoalveolar lavage.

• 대한세포병리학회지
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• 제9권1호
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• pp.1-14
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• 1998

The cytologic distinction of carcinoma cells from reactive mesothelial cells can be difficult, especially in specimens containing abundant reactive mesotheilal cells and inflammatory cells with scant carcinoma cells. This study evaluates the usefulness of mucin and immunocytochemistry for discrimination between reactive mesotheilal cells and carcinoma cells, and sensitivity and specificity of these stains for the detection of metastatic carcinoma in serous effusions. Immunocytochemical panel including mucin cytochemistry with the periodic acid-Schiff(PAS) reaction after or without diastase digestion was undertaken on 127 serous effusion specimens with histologically confirmed diagnoses. The specimens including cell smears and cell blocks were stained with PAS and antibodies to carcinoembryonic antigen(CEA), epithelial membrane antigen(EMA), cytokeratln(CK), and vimentin. The sensitivities of these stains for metastatic carcinoma(127 cases) were 49%(46/94) in PAS, 48%(60/124) in CEA, 89%(97/109) in EMA, 88%(93/106) in CK, and 25%(20/81) in vimentin. The sensitivities of stains for reactive mesothelial cells(36 cases) were 19%(7/36) in EMA, 78%(28/36) in CK, and 75%(27/36) in vimentin. The PAS and CEA stains were not reacted with all cases of benign reactive serous effusions containing abundant reactive mesothelial cells. The specificities of stains for metastatic carcinoma(127 cases) were 100% in PAS, 100% in CEA, 81% in EMA, 22% in CK, and 25% in vimentin. The optimal combination of stains for use in a panel was PAS and CEA. Combined results from these two stains yielded an advanced sensitivity of 8% in PAS and 4% in CEA for metastatic carcinoma. EMA was also cosiderably useful for identification of carcinoma cells. CK and vimentin were not suitable for distinguishing between reactive mesothelial cells and carcinoma cells.

• 한국세라믹학회지
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• 제11권4호
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• pp.37-42
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• 1974

Preparation of pink color stains was studied using manganese sulfate and aluminum salts. As the results obtained in this study, the composition range of the stains showing favorable pink celor was as follows: MnO.0.5-0.8P2O5.1.70-3.00 Al2O3 Furthermore, as the results of applied tests for glazes and the color measured by Color Eye, the usefulness of the stains was approved.

• 대한치과의사협회지
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• 제11권4호
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• pp.271-276
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• 1973

This study is concerned with the effect on Penetration of varing the length of time among the applications of stains, preparations of medicine and radio-active isotope of siver in 120 carious or non carious human teeth with a vital pulp. The study revealed the following conclusions : 1) The stains and preparations penetrated through the dentinal tube and it's seem to be ceased at zone of secondary dentinal area. 2) The stains and preparations did not penetrated in enamel tissues.

• 한국동물학회지
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• 제31권2호
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• pp.133-141
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• 1988

본 연구는 polyacryiamide gel등을 전기영동을 응용, 보존시간에 따른 정액반, 질액반 등에서 PGM$_1$아형의 검출 및 효소활성의 안전성을 조사하여 다음과 같은 결론을 얻었다. (1). 정액반의경우, 실온에서 보존후 7일에는 85%,14일에는 15%의 PGM$_1$아형의 판정이 가능하였고, 21일에는 전혀 판정이 불가능 하였다. (2). 질액반의 경우, 실온에서 보존 후 7일에는 675의 PGM$_1$아형의 판정이 가능하였으나, 14일에는 전혀 불가능 하였다. 한편, 질액에 정액이 혼합된 경우, 질액의 PGM$_1$아형을 판정함으로서, 정액의 PGM$_1$아형의 추정이 가능하였다. 이 결과를 통하여 실제 법생물학 분야에 활용이 가능하다고 인정하였다.

• 대한임상검사과학회지
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• 제37권1호
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• pp.47-55
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• 2005

These studies were done to know decalcification methods to reduce the time of decalcification for quick bone tissue diagnosis. When bone tissue was decalcified with 10 % formic acid at room temperature, decalcification and hematoxylin & eosin (H&E) stains were complete and satisfactory after 12 hours, but some of the tissue sections fell off during staining. In this way, decalcification, H&E stains were complete and satisfactory after 24 hours, 36 hours and 48 hours, tissue sections didn't fall off during staining. When bone tissue was decalcified with 10 % formic acid in a $60^{\circ}C$ paraffin oven, decalcification and H&E stains were complete and satisfactory after 6 hours, but some tissue sections fell off during staining. In this way, decalcification and tissue sections were complete, with no falling off during staining after 8 hours, 10 hours, 12 hours, 14 hours, 24 hours, or H&E stains were satisfactory from 8 hours to 12 hours, but H&E stains appeared to reddish nucleus after 14 hours and 24 hours. Bone tissue was decalcified with 10 % formic acid for 6 hours, 12 hours and 24 hours at DECAL machine frequencies of 15 Hz and 45 Hz, and for 6 hours, 12 hours and 24 hours at a DECAL machine frequency of 90 Hz. Decalcification and H&E stains were complete and satisfactory after 6 hours at the 15 Hz and 45 Hz DECAL settings. Some of the tissue sections fell off during staining at the 15 Hz DECAL machine setting. At the 90 Hz setting, decalcification, H&E stains, and tissue sections were complete and satisfactory with no falling off during staining after 4 hours. In this way, decalcification, H&E stains, and tissue section were complete and satisfactory with no falling off during staining after 12 hours, 24 hours at all machine settings. Bone tissue was decalcified with 10 % formic acid for 6 hours, 12 hours and 24 hours at $37^{\circ}C$ 3 hours, 6 hours and 12 hours at $45^{\circ}C$ and 1 hours, 5 hours and 10 hours at $60^{\circ}C$ with the RHS-1 machine setting at 60Hz. At the temperatures of $37^{\circ}C$, $45^{\circ}C$, and $60^{\circ}C$ decalcification, H&E stains, and tissue sections were complete and satisfactory, with no falling off during staining except for after 6 hours at $37^{\circ}C$. 3 hours, 1 hours, or decalcification, H&E stains, and tissue sections were complete and satisfactory with no falling off during staining after 12 hours and 24 hours at $37^{\circ}C$, 6 hours and 12 hours at $45^{\circ}C$, and 5 hours at $60^{\circ}C$. But H&E stains appeared to reddish nucleus after 10 hours at $60^{\circ}C$. From the above reults, the authors were able to deduce that decalcification is accelerated by heat and frequency. We therefore think that it is necessary for machines which are similar to the RHS-1 machine to be maintained at the temperature evenly with agitation effect for quick decalcification.

• 대한조선학회 특별논문집
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• 대한조선학회 2009년도 특별논문집
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• pp.18-23
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• 2009

After the installation of electric cables at block, PE(pre-erection) and hull stages, the coating stains on the electric cable sheath were unavoidably occurred by additional painting process. According to class rules paint or coating applied on the electric cables shall not adversely affect the mechanical, chemical of fire resistant characteristics of the electric cable sheath. However, there has not been quantitatively studied about the effect of coating stains on properties of sheath materials. In this study, we tried to investigate the effect of coating stains on the performance and deterioration of sheath materials by using FTIR, SEM analysis, flame retardant, high potential voltage and tensile test. The results sowed that coating stains, which were occurred during painting work on site could not adversely affect on the performance and deterioration of sheath materials.

• 보존과학회지
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• 제22권
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• pp.99-108
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• 2008

본 연구는 고구려 벽화고분인 진파리 1, 4호분 벽화의 표면에서 관찰되는 백색과 흑갈색 오염물제거 방안수립을 위해 진행되었으며, 현장 적용실험을 실시하였다. 사전조사에서 금속현미경과 SEM/EDX를 이용하여 백색과 흑갈색 오염물질 시료의 관찰과 성분분석이 실시되었다. 시료에 대한 연구 결과 백색 오염물질은 $CaSO_4$ 혹은 $CaCO_3$로 흑갈색 오염물질은 황산칼슘화합물 혹은 $CaCO_3$와 토양침적물로 추정되며, 백색과 흑갈색 오염물질 제거를 위해 음이온교환수지와 Ammonium bicarbonate를 처리제로 선정하였다. 두 가지 모두 각각의 처리 대상에 대해 양호한 효과를 나타냈으며, 일부 피각형태로 고착화된 오염물질에 대해서는 물리적인 처리법의 병행이 필요한 것으로 확인되었다.

• 한국세라믹학회지
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• 제15권2호
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• pp.66-71
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• 1978

The cobalt blue spinel stains (main composition; CoO:$Al_2O_3$=1 : 1) in CoO-NiO-$Al_2O_$3 and $CoO-Al_2O_3-Cr_2O_3$ system were prepared by the calcination of each component oxides to be adequate for the factory. The color development, the change of the lattice constnat of the spinel and its application to colored glazes were studied. The results were summarized as follows. 1) In CoO-Al_2O_3$ spinel, the excess addition of each component hardly made any variation in lattice constantand alumina-rich spinel specimens caused the brilliant blue color fade. 2) An increase of $Ni^{2+}$ in $CoO-NiO-Al_2O_3$ system, made the lattice constnat of the $CoO-Al_2O_3$ spinel smaller, and an increase of $Cr^{3+}$ in $CoO-Al_2O_3-Cr_2O_3$, larger. 3) Glazed stains under lead glaze were colored nearly same dark blue color fade.