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An Improved Method for DNA Extraction from Paraffin Section Yan-gao Man, Farid Moinfar, Gary L. Bratthauer, Elizabeth A. Kuhls, Fattaneh A. Tavassoli Department.

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Presentation on theme: "An Improved Method for DNA Extraction from Paraffin Section Yan-gao Man, Farid Moinfar, Gary L. Bratthauer, Elizabeth A. Kuhls, Fattaneh A. Tavassoli Department."— Presentation transcript:

1 An Improved Method for DNA Extraction from Paraffin Section Yan-gao Man, Farid Moinfar, Gary L. Bratthauer, Elizabeth A. Kuhls, Fattaneh A. Tavassoli Department of Gynecologic and Breast Pathology, Armed Forces Institute of Pathology ( AFIP ) and American Registry of Pathology ( ARP ), Washington, DC 20306-6000, USA

2 Introduction Technical issues of DNA extraction : ◎ Evaluation of deparaffinization ◎ Satisfied hematoxylin stain ◎ Ratio of cell number to enzyme volume ◎ Monitor digestion process

3 Introduction ◎ Paraffin ( mp 40-60 ℃ ) ◎ Degree of freshness of xylene ◎ Temperature ◎ Duration ◎ Thickness of section Deparaffinization :

4 Introduction Hematoxylin stain :

5 Introduction

6 Introduction ◎ Stable in dissection buffer ◎ Non-lesion on re-cuts ◎ Tissue blocks not accessible ◎ Reducing in 2 % hydrochloric acid ◎ Satisfied both morphological and molecular assessments

7 Introduction Ratio of cell number to enzyme volume : ◎ Larger number of cells  some cell undigested ◎ Larger enzyme volume  low DNA content per unit

8 Introduction ◎ No practical mean to monitor enzymatic digestion process Monitor digestion process :

9 Materials and Method ◎ US 、 Japan 、 China 、 Austria 、 Italy 、 France ◎ Age of the paraffin blocks : 3 months to over 30 years Slide prepare : NameManufactoryNote Microscope slides CMS Slide holders CMS

10 Materials and Method ◎ Thickness : 5-7 μ m ( a few at 10- 12 μ m ) ◎ Clean cutting method : distilled water 、 gloves 、 new blade ◎ Place vertically in 80 ℃ for 30-60 minutes ◎ Cool down 5-10 minutes at room temp. Slide prepare :

11 Materials and Method NameManufactoryNote Xylene Fisher Scientific Ethanol Deparaffinization : ◎ Xylene 3-5 minutes 3 times ◎ Descending concentration of ethanol 3-5 minutes ◎ Running tap water 5 minutes

12 Materials and Method ◎ Hematoxylin 30-60 seconds ◎ Rinse in tap water Stain : NameManufactoryNote Hematoxylin Fisher Scientific Hydrochloric acid Fisher Scientific Ammonium hydroxide LabChem Inc GlycerinCMS

13 Materials and Method ◎ Dip in 2 % hydrochloric acid 3-5 times ◎ Running tap water 5-7 minutes ◎ 1X PBS ( pH7.4 ) contain 1 % ammonium hydroxide 5-7 minutes Stain :

14 Materials and Method ◎ Evaluate the extent of deparaffin :  water retention  hematoxylin stain ◎ Assess hematoxylin stain :  nucleus  cytoplasm ◎ Distilled water 2-3 minutes ◎ 1X PBS contain 10 % glycerin Stain :

15 Materials and Method ◎ Deparaffin ◎ Satisfactory stain for morphology ◎ Microdissection ◎ 2 % hydrochloric acid 3-5 minutes 2 times ◎ 1X PBS ( pH7.0 ) 5-7 minutes ◎ Centrifuge at 2000-3000g 3 minutes ◎ Digestion A Different Approach :

16 Materials and Method NameManufactoryNote Micrometer Olympus Optical 30-Gauge needle Fisher Scientific Mineral oil Fisher Scientific Microcentrifuge tube MJ Research Proteinase K Sigma 10mg/ml ; - 80 ℃ Microdissection & enzymatic digestion :

17 Materials and Method ◎ Microdissection ◎ Digestion buffer :( fresh made )  150 μ l proteinase K + 850 μl mixture  0.5 ml Tween 20 + 0.2 ml 0.5 M EDTA ( pH8.0 ) + 5.0 ml 1 M Tris ( pH8.5 ) + 94.3 ml distilled water Microdissection & enzymatic digestion :

18 Materials and Method ◎ Add digestion buffer  accord number of cells ◎ Mineral oil  equal volume of digestion buffer ◎ 37-40 ℃ 24-48 hours ( magnifier ) ◎ Incubate at 95 ℃ 10 minutes ◎ Store at 4 ℃ Microdissection & enzymatic digestion :

19 Materials and Method Loss of Heterozygosity : NameManufactoryNote LOH marker Research Genetics Gene Amp PCR kit Perkin-Elmer Taq gold DNA polymerase Perkin-Elmer Gel loading buffer Perkin-Elmer DNA size standard Perkin-Elmer Polyacryamide gel Bio-Rad

20 Materials and Method ◎ 30 fluorescent dye-labeled polymorphic DNA markers at 1 、 2 、 3 、 11 、 13 、 16 and 17 ◎ Annealing temperature : 55 - 60 ℃ ◎ 78 to 290 bp ◎ Thermal cycler : Perkin-Elmer ◎ 30 - 40 cycles Loss of Heterozygosity :

21 Materials and Method ◎ 5 – 6 % Polyacryamide Gel ◎ Gel image : Perkin-Elmer 377 DNA sequencer ◎ LOH : 75 % reduction of one allele Loss of Heterozygosity :

22 Materials and Method ◎ DNA markers on exon 1 of the human androgen receptor gene ◎ Hpa Ⅱ : methylation sensitive enzyme ◎ Rsa Ⅰ: control enzyme ◎ Monoclonality : One DNA band or peak after Hpa Ⅱ digestion Clonality analysis : NameManufactoryNote Hpa Ⅱ Gibco/BRL Life Rsa Ⅰ Gibco/BRL Life

23 Results and Discussion ◎ 12 μ m thick human breast No pretreate 80 ℃ 30-60 minutes 1A 放大 1C 放大

24 Results and Discussion ◎ 12 μ m thick human breast No pretreate 80 ℃ 30-60 minutes

25 Results and Discussion No pretreate 80 ℃ 30-60 minutes D16S518 D3S1300 D11S1311  160-300bp TPO  106-130bp

26 Results and Discussion 2 % hydrochloric acid 1 % ammonium hydroxide

27 Results and Discussion ◎ 10 μl digestion buffer : 100-150 cells ◎ Monitoring the digestion process with a magnifier ◎ >24 hours digestion  more concentrated enzyme solution ( 10mg/ml )  re-deparaffinization

28 Results and Discussion

29

30 ◎ Incubation of sections at 80 ℃ for 30-60 minutes ◎ 2 % hydrochloric acid & 1 % ammonium hydroxide ◎ 10 μl digestion buffer : 100-150 cells ◎ Monitoring the digestion process with a magnifier ◎ >24 hours digestion  more concentrated enzyme solution ( 10mg/ml )  re-deparaffinization

31

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33 返回

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