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Human Metaphase Chromosomes & Karyotyping

Human Metaphase Chromosomes & Karyotyping. Chromosome Morphology. Chromosomes are not visible under the light microscope in non-dividing cells (interphase cells).

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Human Metaphase Chromosomes & Karyotyping

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  1. Human Metaphase Chromosomes & Karyotyping

  2. Chromosome Morphology • Chromosomes are not visible under the light microscope in non-dividing cells (interphase cells). • As the cell begins to divide, the threads of chromatin (DNA-protein complex) in the nucleus begin to condense into multiple levels of coiled structures recognizable as chromosomes. • There are two modes of cell division: • Mitosis: is responsible for the proliferation of body (somatic) cells, • Meiosis: is responsible for the production of gametes. • Because mitotic cells are easy to obtain, morphological studies are generally based on mitotic metaphase chromosomes.

  3. Cell division • Cell division can be divided into: • Interphase • Mitosis • Prophase • Metaphase • Anaphase • Telophase • Cytokinesis

  4. Metaphase At metaphase the chromosomes are at their most condensed state, Spindle fibers attaching to the area of the centromere called the kinetochore, forming pole-chromosome fibers.

  5. Anaphase begins with the division of the centromere and the separation of chromatids. Once separated, each chromatid is known as a chromosome. The kinetochore: is the protein structure on chromatids where the spindle fibers attach during cell division to pull sister chromatids apart.

  6. Chromosome Analysis • The best mitotic stage for chromosome analysis is pro-metaphase or metaphase. • A typical metaphase chromosome consists of two arms separated by a primary constriction or centromere. • Each of the two sister-chromatids contains a highly coiled double helix of DNA. • Often the sister chromatids are so close to each other that the whole chromosome appears as a single rod-like structure • A chromosome may be characterized by its total length and the position of its centromere.

  7. Chromosome Number The diploid chromosome number is the number of chromosomes in the somatic cell and is designated by the symbol 2N. The gametes, which have one half the diploid number, have the haploid number N. Thus, there are 23 pairs of chromosomes in human cells.

  8. Of these, 22 pairs are not directly involved in sex determination, and are known as autosomes. The remaining chromosome pair consists of the sex chromosomes, and is directly involved in sex determination. In females the two sex chromosom es are identical (XX), whereas in males the two sex chromosomes are not identical (XY).

  9. Types of Tissue • A variety of tissue types can be used to obtain chromosome preparations. • Some examples include peripheral blood, bone marrow, amniotic fluid and products of conception. • In the case of blood cell culture only cells that are actively dividing can be used for cytogenetic studies. • Normally only white blood cells are used for cytogenetic analysis. • Specific techniques differ according to the type of tissue used.

  10. Overview of Procedure • Collection of blood • Cell culture • Harvesting: stopping the cell division at metaphase • Hypotonic treatment of red & white blood cells • Fixation • Slide preparation • Staining

  11. 1- Collection of blood • Draw 5 ml of venous blood into a sterile heparinized tube containing 0.1 ml of sodium heparin (500 units/ml).

  12. 2- Cell Culture • Sterile technique must be used throughout the cell culture preparation, because it is possible to cause major contamination during this procedure, • 70% of the problems are due to a lack of good sterile technique. • Antibiotics do not eliminate problems of gross contamination which result from poor sterile technique or antibiotic-resistant mutants. • Autoclaving renders pipettes, glassware, and solutions sterile.

  13. 2- Cell Culture Medium • Pipette 10 ml RPMI 1640 medium with L-Glutamine into a 15 ml labeled sterile culture tube • Supplement the medium with the following:

  14. 2- Cell Culture Incubation • Add 1 ml of whole heparinized blood into the tube containing the supplemented medium • Mix contents of tube with gentle inversion • Incubate in 5% CO2 incubator at 37oC for 72 hours

  15. 3- Harvesting • Harvesting: mitotic spindle formation is blocked: usually by adding colcemide to the culture, and the cell division is stopped at the metaphase level. • Pre-warm the Colchicine (0.04 mg/ml) in incubator at 37oC. • Add 25 µl of pre-warmed Colchicine to the culture. • Mix gently and incubate at 37oC for 30-60 minutes. • Note: Colchicine inhibits microtubule polymerization by binding to tubulin, one of the main constituents of microtubules

  16. 4- Hypotonic treatment of red & white blood cells • Centrifuge for 10 minutes at 2000 rpm. • Discard supernatant without disturbing the cells leaving 0.5 ml of fluid. • Add 1 ml of pre-warmed hypotonic solution (0.075 M KCl) at 37oC. • Mix and then add 9 ml of hypotonic solution. • Mix well by Pasteur pipette. • Incubate at 37oC incubator for 17 minutes, • hypotonic solution should not be in contact with cells more than 27 minutes (may cause rupture of WBCs).

  17. 5- Fixation • Fixative must be prepared fresh • Add 3 parts of chilled absolute methanol:1 part glacial acetic acid. • Centrifuge for 10 minutes at 1000 – 1500 rpm. • Remove supernatant leaving about 0.5 ml of fluid on top of cells. • At this time there is probably a small whitish or reddish film at the bottom of the tube. • The film contain red blood cell debris and enlarged WBCs.

  18. 5- Fixation • Add 5 ml of fixative to the tube. • Mix with a Pasteur pipette 3-4 times. • Place in refrigerator for 30 minutes. • Centrifuge the tube for 10 minutes at 1000-1500 rpm. • Remove supernatant and add another 6 ml of cold fixative, & mix well. • Centrifuge the tube for 10 minutes at 1000-1500 rpm. • Repeat the last two steps. • Remove the supernatant leaving 1 ml of fluid at the bottom. • The remaining material will be used to make the slides.

  19. 6- Slides Preparation • The slide must be exceptionally clean • Lay slides on a paper towel • Withdraw a few drops of cell suspension into a pipette • From a height of 20 cm, drop 2 or 3 drops of fluid on each slide • Allow the slides to dry

  20. 7- Staining • Stain the slides by immersion in fresh Giemsa stain for 7-10 minutes • Remove slides from stain & rinse in distilled water • Observe under microscope 40X then under oil immersion

  21. Karyotyping

  22. What is a Karyotype? • A display or photomicrograph of an individual’s somatic-cell metaphase chromosomes that are arranged in a standard sequence (usually based on number, size, and type)

  23. Why do scientists look at chromosomes? • Scientists can diagnose or predict genetic disorders by looking at chromosomes. • This kind of analysis is used in prenatal testing and in diagnosing certain disorders, such as • Down syndrome, • or in diagnosing a specific types of leukemia.

  24. Chromosome abnormalities • Chromosome abnormalities can be • numerical, as in the presence of • extra • or missing chromosomes • Structural as in translocations, inversions, large scale deletions or duplications.

  25. Chromosomal Abnormalities • Alterations in chromosome number. • Euploid - normal set (2n) • Polyploidy – extra set of the entire genome. (3n, 4n, ……….etc) • Aneuploidy – the number of chromosomes is not a multiple of the normal haploid number. • Monosomy • one member of a chromosome pair is missing, (2n-1) • Trisomy • one chromosome set consists of 3 copies of a chromosome, (2n+1)

  26. Turner syndrome results from a single X chromosome (45, X or 45, X0). Klinefelter syndrome, the most common male chromosomal disease (47, XXY) Down syndrome, a common chromosomal disease, is caused by trisomy of chromosome 21.

  27. Chromosomal abnormalities (can be detected by karyotyping)

  28. Chromosomal abnormalities (can be detected by karyotyping) Philadelphia Chromosome - CML

  29. Situations where analysis is strongly recommended • Problems with early growth & development • Fertility problems • Neoplasia • Pregnancy in older women

  30. How Do Scientists Identify Chromosomes? • Three key features to identify their similarities and differences: • Size. This is the easiest way to tell two different chromosomes apart. • Banding pattern. The size and location of Giemsa bands on chromosomes make each chromosome pair unique. • Centromere position. Centromeres are regions in chromosomes that appear as a constriction. • Using these key features, scientists match up the 23 pairs

  31. In metacentric chromosomes, the centromere lies near the center of the chromosome.Submetacentric & very Submetacentric chromosomes, have a centromere that is off-center, so that one chromosome arm is longer than the other. In acrocentric chromosomes, the centromere resides very near one end.

  32. Chromosome banding • Chromosomes are stained with various dyes enabling the chromosome segments to be identified • Most methods can distinguish 550 bands/ haploid set • High resolution methods can distinguish up to 850 bands/ haploid set that can allow identification of small interstitial deletions

  33. G-Banding • Regions that stain as dark G bands replicate late in S phase of the cell cycle and contain more condensed chromatin, • While light G bands generally replicate early in S phase, and have less condensed chromatin.

  34. The difference between dark- and light-staining regions was believed to be caused by differences in the relative proportions of bases: • G-light bands being relatively GC-rich • G-dark bands AT-rich

  35. Chromosome Groups

  36. Overview of Procedure • Collection of blood • Cell culture • Stopping the cell division at Metaphase • Hypotonic treatment of red & white blood cells • Fixation • Slide preparation • Slide dehydration • Treatment with enzyme • Staining

  37. 7- Slide dehydration • Place fixed, dry slides on slide rack in 60oC oven • Bake for 3 days • Allow to cool before proceeding to the next step

  38. 8- Treatment with enzyme • Prepare 0.025% trypsin solution fresh, by mixing 5 ml of 0.25% trypsin with 45 ml Hank’s solution • Immerse slide in 0.025 % trypsin for 10-120 seconds • Remove slide from trypsin and immediately immerse in phosphate buffer to stop trypsin action

  39. 9- Staining • Prepare a dilution of Giemsa stain by mixing 1 part of Giemsa stain with 3 parts of Phosphate buffer • Flood slide with Giemsa stain for 2 minutes • Rinse slides thoroughly with distilled water • Allow slides to drain, then place on 60oC slide warming tray until completely dry

  40. 21 22 x y

  41. Exercise

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