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Methods of Sample Preparation

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Presentation on theme: "Methods of Sample Preparation"— Presentation transcript:

1 Methods of Sample Preparation
Preparation of Cells/Tissues for Microscopy

2 Methods of Preparation
Fresh cells and tissues Cytological techniques Sectional methods Sample preparation for the microtome sectioning

3 1. Fresh cells and tissues
Direct examination Isotonic solution (saline) (e.g. subcutaneous connective tissue)

4 1. Fresh cells and tissues
Direct examination Smear Cells suspended in fluid (e.g. blood, urine or lymph)

5 1. Fresh cells and tissues
Direct examination Smear Dissociation / teasing Thick tissue

6 1. Fresh cells and tissues
Direct examination Smear Dissociation / teasing Natural state (^^) but lack of contrast (TT) Specialized microscopy (e.g. Phase-contrast microscopy) Vital staining

7 Vital Staining stain that can be applied on living cells without killing (fixing) them technique in which a harmless dye is used to stain living tissue for microscopical observation neutral red, Janus green B, eosin Y, brilliant cresyl blue, nigrosin, Bismarck brown, crystal violet, methylene blue & food color

8 Vital Staining stain that can be applied on living cells without killing (fixing) them technique in which a harmless dye is used to stain living tissue for microscopical observation Supra-Vital Staining the living tissue may be removed directly and subsequently stained Intra-Vital Staining injection of dye into the living organism and the stained tissue removed and examined Higher concentrations of vital stain will kill the cell only certain cytoplasmic elements can be demonstrated

9 2. Cytological techniques
widely applied to the diagnosis of disease Cells obtained from all parts of body by Fine needle aspiration (FNA) technique Exfoliative cytology Impression method

10 Fine needle aspiration cytology

11 Exfoliative cytology the analysis of cells shed from the body (e.g. Pap smear) Harvest Exfoliative Cells from the normal tissue

12 Pap smear to detect cancerous or precancerous conditions of the cervix
George N. Papanicolaou (1943)

13 Impression cytology pressing a clean glass slide firmly against the surface of the organ or tissue and then lifting it away

14 2. Cytological techniques
widely applied to the diagnosis of disease Cells obtained from all parts of body by Fine needle aspiration (FNA) technique Exfoliative cytology Impression method Smear, Fix and Stain 2D-, flattened larger than the same cells in tissue sections Cellular details are more easily seen

15 3. Sectional methods Why Section? Microtome Cryostat
Cutting the specimen into very thin translucent slices or sections Microtome Cryostat Why Section? Tissues and organs are usually too thick for light pass through them.

16 Sample preparation for the microtome sectioning
formaldehyde ethanol xylene paraffin (70% → →100%)

17 Paraffin embedded tissue block

18 Microtome 1-10 μm thick For sectioning paraffin-embedded tissues

19

20

21

22 Ultramicrotome For TEM sections less than 1μm thick Resin-embedding
glass or diamond knife

23 Cryostat Freezing microtome Fixed by Rapid freezing
For the frozen block of tissue Sample preparation Fixed by Rapid freezing In Isopentane or liquid nitrogen Support medium (e.g. OCT) -20 ± 5 ℃ Control panel Freezing chamber (Cutting Chamber) Handle

24 Why cryostat? Advantages of Frozen sections
Rapid preparation of sections Better for the demonstration of histochemically sensitive molecules enzymes lipids Superior for the preservation of antigenicity

25 Disadvantages Quality of sections
Inferior to paraffin sections Less stable than paraffin- or resin-embedded sections Inconvenient storage Low temperature cabinet or a jar of fixative at room temperature not ideal method for very thin section (1-3 μm)

26 ice crystal artifacts (in cryostat)

27 Problems in the study of sections
Structures seen microscopically may differ from the structures present when they were alive (=artifacts) Shrinkage (by the fixative, ethanol or heat), Wrinkles and so on Three-dimensional structures appear to have only two dimensions in thin sections.

28 knife scratches & splitting

29 Shrinkage

30 Wrinkles

31 Poor fixation

32 Problems in the study of sections
Structures seen microscopically may differ from the structures present when they were alive (=artifacts) Shrinkage (by the fixative, ethanol or heat), Wrinkles and so on Three-dimensional structures appear to have only two dimensions in thin sections.

33 3-D structures in 2-D sections

34

35

36 Serial sections Serial sections and reconstructing the images 3- dimensionally provides better understanding

37 Learning Resources Junqueira’s Basic Histology ; pp 1-3
Looking at the Structure of Cells in the Microscope

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