Pages

Thursday, June 3, 2010

Mouse (mus musculus) intestine





Cross-section of the small intestine of mouse (mus musculus) close to the duodenum. The lumen of the gut is at the top of each image. The first and last images were taken at 100x while the second and third showing villi of the epithelium lining the gut at 400x. Purple dots in the middle of each cell are the nucleus of each epithelial cell and pink is the cytoplasm of each cell.
The slide was prepared at the lab of the university, as part of a practical session, but the pictures were taken using my personal light microscope at home with a regular camera.

Wednesday, June 2, 2010

Onion Skin







Onion skin cells alignment at 100x.
Pictures were taken with my digital camera using my personal light microscope at home.

Tuesday, June 1, 2010

Immuno-histochemistry and In-situ Hybridization





Both pictures show mouse (mus musculus) embryos 9.5days old and 11.5d respectively.
In the top picture the embryo was hybridized using the anti-sense probe for FGF8 and detected by alkaline phosphatase conjugated antibodies which stained the specific sites of expression of FGF8. The areas in which the staining is more intense are the midbrain hindbrain boundary, forelimb bud and hindlimb bud, especially the edge of the hindlimb bud, the apical ectodermal ridge.
In the second picturethe embryo that was incubated with both primary antibodies and secondary conjugated with peroxidase antibodies, showing the specific sites of expression of neurofilaments. The visible staining represents neurofilaments, spinal ganglia (SpG) developing in the developing vertebrae and the developing cranial nerves, the vagus neurofilament, the glossopharyngeal (GlPh) neurofilament and the hypoglossal neurofilament.

Both pictures were taken from a camera connected to a dissection microscope.

Immunofluorescence




The green fluorescence represents the location in the cell of a protein found in the Golgi apparatus in all pictures.
The red fluorescence:
1) in the top picture represents the location of the cytoskeleton of the cell and specifically microtubules (anti-β-tubulin used)
2) Middle picture represents the location of late endosomes and lysosomes in the cell (anti-CD63 used)
3) in the bottom picture represents the location of the endoplasmic reticulum (E.R.) in the cell (anti-PDI used).

The cells used were COS-7 (African green monkey SV40 transformed kidney fibroblasts) and confocal microscopy was used to view the fluorescence emitted by the fluorophore of different color conjugated to secondary antibodies.

Haemoglobin Studies



Haemoglobin from horse red blood cells was purified, some was left to crystallize using different salt concentrations (top picture) and a sample was loaded on a polyacrylamide gel along with molecular weight markers. Sodium Dodacyl Sulfate - Polyacrylamide Gel Electrophoresis (SDS-PAGE) is a very useful technique for all bio-science researchers, giving relatively a lot of information about a protein (especially the 2-D gel).