以三倍頻顯微術觀察並辨別白血球細胞

Shi-Hong Huang; 黃仕泓

請用此 Handle URI 來引用此文件： http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/55404

完整後設資料紀錄

DC 欄位	值	語言
dc.contributor.advisor	劉子銘(Tzu-Ming Liu)
dc.contributor.author	Shi-Hong Huang	en
dc.contributor.author	黃仕泓	zh_TW
dc.date.accessioned	2021-06-16T04:00:40Z	-
dc.date.available	2018-02-03
dc.date.copyright	2015-02-03
dc.date.issued	2014
dc.date.submitted	2014-10-31
dc.identifier.citation	[1] Goldman L, and Schafer AI, “Mechanisms of inflammation and tissue repair., ” 24th edition, chapter 47. [2] Kolaczkowska E, and Kubes P, “Neutrophil recruitment and function in health and inflammation.,” Nature Reviews Immunology, 13(3), 59-75, 2013 Mar. [3] Frederic Geissmann, Markus G. Manz, Steffen Jung, Michael H. Sieweke, Miriam Merad,and Klaus Ley, “ Development of monocytes, macrophages and dendritic cells.,” available in PubMed Comprises, 2011 February 5. [4] Alberts B, Johnson A, and Lewis J, “Molecular Biology of the Cell.,” 4th edition, chapter 24. [5] MA Lichtman, E Beutler, TJ Kipps, U Seligsohn, K Kaushansky, and JT Prchal, “Williams Hematology.,” 7th edition. [6] Teerasaksilp S, Wiwanitkit V, and Lekngam P, “Comparative study of blood cell staining with wright-giemsa stain, field stain, and a new modified stain.,” Lab Hematol, 11(1), 76-8, 2005. [7] Shapiro, H.M, “Practical Flow Cytometry.,” 3rd edition Wiley-Liss. [8] Ormerod, M. G., “Flow Cytometry.,” 3rd edition. [9] J. Paul Robinson, 'Comparative Overview of Flow and Image Cytometry.,' Current Protocols in Cytometry, 12.1.1-12.1.11, 2005. [10] D Lanigan, P A McLean, B Curran, and M Leader, ' Comparison of flow and static image cytometry in the determination of ploidy.,' Journal of Clinical Pathology , 46, 135-139, 1993. [11] Michael Brown, and Carl Wittwer, 'Flow Cytometry: Principles and Clinical Applications in Hematology.,' Journal of Clinical Pathology, 46, 135-139, 1993. [12] Natasha S. Barteneva, Elizaveta Fasler-Kan, and Ivan A. Vorobjev, ' Imaging Flow Cytometry: Coping with Heterogeneity in Biological Systems.,' Journal of Histochemistry & Cytochemistry, 60(10), 723-733. [13] David A. Basiji, William E. Ortyn, Luchuan Liang, Vidya Venkatachalam, and Philip Morrissey, ' Cellular Image Analysis and Imaging by Flow Cytometry.,' available in PubMed Comprises, 2008 September 1. [14] Pozarowski P, Holden E, and Darzynkiewicz Z, ' Laser scanning cytometry: principles and applications.,' Methods in Molecular Biology, 319, 165-92, 2006. [15] J. G. Fujimoto, D. Huang, E. A. Swanson, C. P. Lin, J. S. Shuman, W.G. Stinson,W. Chang, M. R. Hee, T. Flotte, K. Gregory, and C. A.Puliafito, “Optical coherence tomography.,”Science, Vol.254 , 1178-1181, Nov.1991 [16]B. E. Bouma, G. J. Tearney, “Handbook of Optical Coherence Tomography.,” Marcel Dekker, Inc., 2002. [17] Denk W., Strickler J. H., Webb W. W., “Two-photon laser scanning fluorescence microscopy., ” Science, 248, 73-6, 1990. [18] Chi-Kuang Sun, Shi-Wei Chu, Szu-Yu Chen, Tsung-Han Tsai, Tzu-Ming Liu , Chung-Yung Lin , and Huai-Jen Tsai “Higher harmonic generation microscopy for developmental biology.,” Journal of Structural Biology, 147, 19-30, 2004. [19] Born M, and Wolf E., “Principles of Optics.,” Cambridge University Press, England, 1999. [20] Robert H Webb., “Confocal optical microscopy.,” Reports on Progress Physics, 59(3), 427-471, 1996. [21] F. Nicoud, and T. Poinsot, “Thermoacoustic instabilities: Should the Rayleigh criterion be extended to include entropy changes?,” Combustion and Flame 142, 153–159, 2005. [22] Minsky M., “Microscopy Apparatus., ” U.S. Patent, No. 3, 013-467, 1957. [23] P. Tijriik, , and T. Wilson, “Full length article Rigorous theory for axial resolution in confocal microscopes.,” Optics Communications, I37, 127- I35, 1997. [24] H. A. Haus, “Waves and Fields in Optoelectronics.,” Prentice Hall, 1984. [25] Franken P. A., Hill A. E., Peters C. W., and Weinreich G., “Generation of Optical Harmonics”, Physical Review Letters, 7(4), 118-119, 1961. [26] J. F. WARD, “Calculation of Nonlinear Optical Susceptibilities Using Diagrammatic Perturbation Theory. ”, reviews of modern physics, 1965 January. [27] R. W. Boyd, “Nonlinear Optics. ”, Academic Press, 1992 [28] Ho-Che Kuo, “Monitoring Thermally Induced Alteration of Collagen by SHG.,” National Sun Yat-Sen University, 2005 [29] Diana Jeong, “Second Harmonic Generation in Nonlinear Optical Crystal., ” [30] Loaiza and Dood, “ Second-Harmonic Generation., ” Leiden University. [31] Ward JF, and New GHC,“Optical third harmonic generation in gases by a focused laser beam.,” Physical Review, 185-57, 1969. [32] Born M, and Wolf E, “Principle of Optics.,” 7th edition, Cambridge University Press, 1999 [33]Barad Y, Eisenberg H, Horowitz M , and Silberberg Y, “Nonlinear scanning laser microscopy by third-harmonic generation.,” Applied Physics Letters, 70-922, 1997. [34] Centonze V. E., and White J. G., 'Multiphoton excitation provides optical sections from deeper within scattering specimens than confocal imaging.,' Biophysical Journal, 75, 2015-24, 1998. [35] Sako Y., Sekihata A., Yanagisawa Y., Yamamoto M., Shimada Y., Ozaki K., and Kusumi A., 'Comparison of two-photon excitation laser scanning microscopy with UV- confocal laser scanning microscopy in three-dimensional calcium imaging using the fluorescence indicator Indo-1.,' Journal of Microscopy, 185, 9-20, 1997. [36] Mandy FF, Bergeron M, and Minkus T, “Principles of flow cytometry.,” Transfusion Science, 16, 303-14, 1995. [37] Michael Brwon, and Carl Wittwer, “Flow Cytometry: Principles and Clinical Applications in Hematology.,” Clinical Chemistry, 1221–1229, 2000. [38] Watson JV, “he early fluidic and optical physics of cytometry.,” Cytometry, 38, 1-14, 1999. [39] Nicole Y.L. Lam, Timothy H. Rainer, Rossa W.K. Chiu, and Y.M. Dennis Lo, “EDTA Is a Better Anticoagulant than Heparin or Citrate for Delayed Blood Processing for Plasma DNA Analysis.,” Clinical Chemistry ,50, No. 1, 2004. [40] M. Mohri, and H. Rezapoor, “Effects of heparin, citrate, and EDTA on plasma biochemistry of sheep:Comparison with serum.,” Research in Veterinary Science, 86, 111-114, 2009.
dc.identifier.uri	http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/55404	-
dc.description.abstract	血液是醫療檢查中重要的評鑑指標，紅血球、白血球和血小板的組成比例與數量都有其健康意涵，醫院對於血液的分析，多以抽血方式，再經由流式細胞儀等分析儀器進行樣本分析，此屬侵入式醫療行為，不只對受測者帶來心理負擔，也易讓抽離體外的檢體因外在因素而變質，進而影響判讀之正確性，未來，我們希望利用非線性光學顯微術，以非侵入式檢測對各類血球統計與分析，解決現有問題。為達此弘遠目標，本研究扮演開山始祖的角色，著重血球在非線性光學下的特徵差異與辨識條件，因非線性光學顯微術具有次微米等級三維空間解析能力，可做深層光學成像，不具生物傷害性，且不需經由染劑標定，省去染劑標定可使血球更近於真實樣貌，本研究利用摻鉻貴橄欖石晶體雷射做為激發光源，擷取受測物所發出的倍頻訊號，經由FPGA(ALTERA DE4)將類比訊號轉為數位訊號且擷取影像，最後由Visual Studio撰寫出的影像軟體，成像與影像優化，並利用此系統觀察血球的各項特徵。在三倍頻的成像下，紅血球與血小板有很強的三倍頻訊號，因尺寸差異很容易將兩者辨別，白血球三倍頻訊號較弱，主要又可分成中性粒細胞(Neutrophil)、淋巴球(Lymphocyte)、單核球(Monocyte)，在影像特徵下，中性粒細胞比淋巴球、單核球三倍頻訊號更強，細胞內有多個小核體，也常出現明顯細胞膜結構，淋巴球細胞最小，細胞內有一大圓核，且細胞內常出現一圓形亮點，單核球細胞最大，細胞核不規則狀，影像特徵可以輔助辨識，但為達更快速的辨別，我們以細胞大小、三倍頻強度和自體紅螢光強度做為辨別條件，三倍頻強度以中性粒細胞最強，單核球、淋巴球無顯著差異，自體紅螢光強度依然為中性粒細胞最強，單核球居次，淋巴球最弱，透過這些差異可有效將三類白血球分成三群。雖目前成果離非侵入式活體血球辨識仍有段差距，但本研究結果可輔助流式細胞儀對血球的分選，流式細胞儀常為達更高的辨別正確性，使用染劑的添加，但染劑的添加不只經費負擔，對細胞的變異也存在風險，利用本研究結果，不僅可增加流式細胞儀對血球細胞的篩選條件，並可提供影像的特徵辨別，讓分選正確率再次提升。	zh_TW
dc.description.abstract	Blood is an important index of medical examination. The percent composition of red blood cells, white blood cells and platelets in blood is related to health. In the hospital, drawing blood has been a dominant way of health exam. The method is an invasive medical practice, and vitro specimen tends to be affected by the external factors, which is possible to affect the accuracy of the estimation. To overcome the problems mentioned, we use nonlinear optical microscopy to gather statistics and analysis of all types of blood cells with non-invasive detection in the future. My research focuses on the differences of characteristics of blood cells observed by nonlinear optical microscopy and broadening the conditions of identification. Equipped with sub-micron grade three-dimensional analysis, non-linear optical microscopy can be applied to get deep optical images and causes no biological damages. In addition, no dye is included in the research, so the blood cells remain almost intact. In the research, we use Cr:forsterite laser as the excitation source and further to collect THG signals emitted by target objects. Then, we capture the images generated by the transition from analogical signals to digital signals processed by the FPGA (ALTERA DE4). Finally, the optimized images, generated by an image software (programmed by visual studio) are adopted to observe the characteristics of blood cells. In the third harmonic generation images, the red blood cells and platelets show a strong third harmonic generation signal. It is easy to identify them because of the size difference between the two. As for Leukocyte, it can be further divided into three types: neutrophil, lymphocyte and monocyte. Unlike red blood cells and platelets, the THG signal of Leukocyte is weaker. Because of the characteristics observed from optimized images, we can easily identify the specific type of Leukocyte. It is observed that neutrophil THG signal is stronger than lymphocyte and monocyte. Neutrophil has multiple small nucleus, and the cell membrane structure is obvious. In terms of the size of lymphocyte, it is the smallest and its circle nuclear is bigger, and oftentimes, it can be identified because of a circular bright spot. Monocyte, being the largest in size, has an irregular-shaped nuclear. Because of the optimized images, identification of cells become easy. In order to achieve more rapid identification. The size of cells, and the intensity of THG and the intensity of fluorescence condition identification of specific types of cells. In terms of the intensity of THG, Neutrophil exhibits the strongest, while monocyte and lymphocyte shows no significant difference. Concerning the intensity of fluorescence, neutrophil exhibits the strongest and lymphocyte the weakest. With the distinctive features of cells mentioned above, the three types of white blood cells can be effectively identified and further divided into three groups. Although much remains to be done, but this study is still valuable in that the empirical results enable the flow cytometry to sort blood cells effectively. Sorting blood cells through flow cytometry is usually conducted with dye; the use of dye is consuming and the most importantly, it is possible to cause cell mutation. With the result of this study, the broadened conditions on blood cells sorting conducted by flow cytometry and the features observed by the optimized images surely improve the accuracy of blood cells sorting.	en
dc.description.provenance	Made available in DSpace on 2021-06-16T04:00:40Z (GMT). No. of bitstreams: 1 ntu-103-R01548048-1.pdf: 2690248 bytes, checksum: df6b517419c9d47658667b988662a1ec (MD5) Previous issue date: 2014	en
dc.description.tableofcontents	致謝 I 中文摘要 III Abstract V 目錄 VII 第一章緒論 1 1.1血液檢驗在臨床之重要性 1 1.2血液檢驗 2 1.3流式細胞儀的演進 3 1.4影像流式細胞掃描儀 5 1.5光學影像技術的運用 7 第二章基礎理論 10 2.1傳統光學顯微鏡 10 2.2共軛焦顯微術 13 2.3非線性光學顯微術 16 2.3.1二倍頻(Second-Harmonic Generation，SHG) 17 2.3.2三倍頻(Third-Harmonic Generation，THG) 20 2.3.3多光子影像技術 22 2.4輔助流式細胞儀辨識技術 24 2.5流式細胞儀(Flow Cytometry)原理 25 第三章實驗架構與研究方法 29 3.1光學系統 29 3.1.1雷射 29 3.1.2光路 30 3.1.3掃描儀 31 3.1.4反射(螢光)穿透(三倍頻) 32 3.1.5資料擷取 33 3.1.6雷射訊號與FPGA同步機制 33 3.2影像系統 34 3.2.1取像介面 34 3.2.2影像修正 35 3.3白血球純化萃取 37 3.4樣本固定與觀測 39 3.5數據分析 40 第四章實驗結果與討論 42 4.1紅血球、白血球、血小板形態差異 42 4.2 EDTA與肝素對血球之影響 43 4.3流式細胞儀對血球細胞的影響 45 4.5白血球辨別方法 54 4.6結果驗證 61 4.7結果討論 66 第五章結論與未來展望 74 第六章參考文獻 76
dc.language.iso	zh-TW
dc.subject	流式細胞儀	zh_TW
dc.subject	中性粒	zh_TW
dc.subject	單核球	zh_TW
dc.subject	淋巴球	zh_TW
dc.subject	倍頻顯微術	zh_TW
dc.subject	Lymphocyte	en
dc.subject	Neutrophil	en
dc.subject	Monocyte	en
dc.subject	Flow Cytometry	en
dc.subject	Harmonic Generation	en
dc.title	以三倍頻顯微術觀察並辨別白血球細胞	zh_TW
dc.title	Using Third Harmonic Generation Microscopy to Observe and Identify The Type of Leukocytes	en
dc.type	Thesis
dc.date.schoolyear	103-1
dc.description.degree	碩士
dc.contributor.oralexamcommittee	朱士維(Shih-Wei Chu),王宗道(Tsung-Tao Wang)
dc.subject.keyword	中性粒,單核球,淋巴球,倍頻顯微術,流式細胞儀,	zh_TW
dc.subject.keyword	Neutrophil,Monocyte,Lymphocyte,Harmonic Generation,Flow Cytometry,	en
dc.relation.page	79
dc.rights.note	有償授權
dc.date.accepted	2014-10-31
dc.contributor.author-college	工學院	zh_TW
dc.contributor.author-dept	醫學工程學研究所	zh_TW
顯示於系所單位：	醫學工程學研究所

文件中的檔案：

檔案	大小	格式
ntu-103-1.pdf 未授權公開取用	2.63 MB	Adobe PDF

顯示文件簡單紀錄

系統中的文件，除了特別指名其著作權條款之外，均受到著作權保護，並且保留所有的權利。