Anti-Piscirickettsia salmonis monoclonal antibody. Product no: P05

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Anti-Piscirickettsia salmonis monoclonal antibody Product no: P05

Product Description The monoclonal antibody (Mab) against Piscirickettsia salmonis is specific for this bacterium. The specificity of the Mab has been tested against a range of bacterial and viral pathogens that infect fish (see product information at www.aquaticdiagnostics.com). The Mab is of an IgM isotype.

Use of product The Mab is recommended for use in immunohistochemistry (IHC), but can also be used in IFAT. The optimal conditions for use of this product vary depending on the procedure used. The user must determine the suitability of the product for a particular procedure. This product is for in vitro use only. Vial Contents Each vial contains 200 μg of lyophilised protein prepared from bovinefree culture medium and contains no animal-derived stabilisers. This is sufficient for between 100-200 tests depending on the area of tissue to be screened in IHC. The product should be reconstituted as follows: Add 1 ml of phosphate buffered saline (PBS) (see buffers) to the vial and store as aliquots. Dilute 1/10 in PBS before use. Storage Store at -20 C or below prior to reconstitution. For prolonged storage, the Mab solution should be stored at -20 C, or below. Repeated freeze thawing of the product should be avoided.

Suggested protocol for the detection of Piscirickettsia salmonis in fixed tissue sections by immunohistochemistry This procedure has been developed to work on tissues fixed in 10% buffered formalin for 24 hours. Individual protocols may have to be developed depending upon the tissue examined, fixation etc. Procedure - Prepare paraffin-embedded tissue sections. - Dewax and rehydrate sections in xylene (2 x 5min), 100% ethanol (5 min), 70% ethanol (3 min), then rinse in distilled water. - Place slides in a humid chamber. - Keep sections moist at all times - do not allow them to dry out. - Mark rings around the tissue sections using a wax PAP pen. - Block endogenous peroxidase activity by incubating the slides for 10 min at room temperature ( 22 C) with H 2 O 2 in methanol (see buffers). - Wash the slides three times with Tris buffered saline (TBS) (see buffers). - Block non-specific binding sites with normal goat serum diluted 1/10 in TBS for 10 min at room temperature. - Pour off the serum and remove excess serum tapping the slide edges on a paper towel. - Place 50-100 μl of reconstituted anti-p. salmonis Mab onto the tissue sections (the volume added will depend on the size of sample to be covered) and incubate for 60 min at room temperature in a humid chamber. - Use appropriate controls i.e. known positive tissue as a positive control and uninfected tissue as a negative control; these should both be incubated with the reconstituted Mab and PBS separately. - Wash slides three times with TBS. - Add goat anti-mouse IgM-biotin conjugate (1/100 in TBS) to the slides for 30 min [NB some commercial anti-mouse IgG-biotin conjugates cross react with mouse IgM]

- Wash slides three times with TBS - Add streptavidin- horseradish peroxidase (1/100 in TBS) to the slide for 30 min - Wash slides three times with TBS - To visualise the reaction, incubate the slides for 10 min with DAB solution (see buffers) or with a commercially available True Blue staining kit following the manufactures instructions. - If stained with DAB stop the reaction by immersing the slides in tap water and counter-stain them with haematoxylin for 3-4 min. - Rinse in tap water for 10 min. - Dehydrate the slides in 70% ethanol (3 min), 100% ethanol (5 min), xylene (2 x 5 min) - Mount the slides with Pertex and leave in fume cupboard to set. - Examine tissue under a light microscope cells infected with the bacterium appear golden brown in colour when stained with DAB. Buffers Phosphate buffered saline (PBS) 0.02M Phosphate, 0.15M NaCl ph adjusted to 7.2 with HCl NaH 2 PO 4.2.H 2 O 0.876g Na 2 HPO 4.2.H 2 O 2.56g NaCl 8.77g Tris buffered saline (TBS) Trisma base 2.42g NaCl 29.24g

Dissolve in approximately 900 ml distilled water, adjust ph to 7.2 using HCl and make up to 1 litre 10% (v/v) Hydrogen peroxide in methanol Add 1ml H 2 O 2 (30% v/v solution) to 9 ml methanol 3,3 -Diaminobenzidinetetrahydrochloride (DAB) Dissolve one 10mg tablet DAB in 6.67mls TBS Place 0.5 ml aliquots of the solution into bijoux bottles, store at -20 C. For use add 5mls TBS and 0.1ml 1 % H 2 O 2 to 0.5 ml aliquot NB. DAB is a possible carcinogen

Certificate of Analysis Anti Piscirickettsia salmonis monoclonal antibody Product no. P05 Batch no. Date of expiry Activity in IHC: Cells infected with the bacterium appear golden brown in colour when stained with DAB.

Aquatic Diagnostic Ltd., Institute of Aquaculture, University of Stirling, Stirling, Scotland, FK9 4LA Telephone: +44 (0)1786 466568 Fax: +44 (0)1786 472133 E-mail: aquaticdiagnostics@stir.ac.uk http://www.aquaticdiagnostics.com