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> First-Class Program Evaluation Form The First Class Program Your purchase order reference: EGT Quotation Number: Antibodies that work in your application, guaranteed > Custom peptide antibodies adapted to VAT Nr. : If VAT exempt please include a copy of certificate DELIVERY ADDRESS INVOICE ADDRESS (Please fill in delivery information if different from invoicing information) Institute/Company: Institute/Company: Department/Lab.: Department/Lab.: Contact Person: Contact Person: Address: Address: your application > B-Epitopes are selected based on the antigen’s predicted 3D structural Postal Code: features in your application conditions Country: Country: Phone: Phone: Fax: Fax: e-mail: e-mail: > The right antibody for your immunoassay or your money back We have improved antigenic sequence prediction algorithms The antigenic surface of a protein is a 3-D patchwork of small linear antigenic sequences. Individually, each sequence is antigenic but, depending on the number of accessible residues in the interaction, the affinity will be either acceptable or too low. Currently, antibody affinities of 10-8 to 10-9 M can be expected for linear epitope, by calculating and analyzing the structure of each potential epitope. We will propose the most appropriate antigenic fragments that should exhibit such affinities. Ref: PRO-FIRSTCLASS-0207-V2 An epitope for each application As the structure of your protein may vary with each assay, an assay–antigen specific analysis must be made to determine structural and interaction properties. Major factors leading to changes in the epitope structure are (1) denaturation by detergent and (2) chemical modification of the amino acids of the epitope, for example with fixatives or other chemicals. For your immuno-assay technique the most exposed epitope may not be your best choice. Depending on whether the antibody will be used on a native, a detergent-denatured or a fixative-modified structure of your protein, we shall select either a flexible or a more rigid region of the protein such as a turn or a helix. Increased flexibility is reported to lead to improved affinity, however, rigid structures can provide good epitopes more resistant to detergent denaturation. Additionally, sequences containing aromatic residues rather than highly polar amino acids may be selected if application conditions will involve the use of chemicals that react with polar moieties. Indeed, as long as they do not impair the fragment accessibility, hydrophobic residues could improve the affinity. The prediction of the best epitope is closely linked to the application for which the antibody will be used. The “First Class” program – what do we do? Using a consensus of epitope prediction procedures we characterize all potential linear epitopes. Then, in a second step, we calculate their structures and keep those whose characteristics are adequate to raise high affinity antibodies. In the third step, we select the fragment(s) that are the most likely to be useful in your immuno-assay. What do we need ? The accession number of the protein of interest and a complete description of the application in which you will use the antibody. Please complete the questionnaire on the reverse side. We include • • • • • • • • • • Application specific peptide design 5 pre-immune rabbit sera for animal selection Synthesis of 2 peptides, 20-25 mg each Coupling of each peptide to a carrier protein Double X protocol in a 4-month program ELISA testing to monitor titer evolution Affinity purification of 5 ml of serum against each peptide Delivery of 15 - 20 mg of free peptide Remaining antisera All shipping costs City: Postal Code: Protein accession #: 1. For which experimental method do you want a guarantee? (only one technique please) [email protected] • [email protected] • www.eurogentec.com 5. Is your protein a membrane protein Yes ELISA in the absence of detergent or fixative Western Blot Immunoprecipitation with no detergent Immunoprecipitation in the presence of detergent Specify the concentration and the name of the detergent ………………………………………………………………...........…………………… Staining of chemically fixed tissues Specify the fixative ……….....................................……………...…… Staining of frozen-fixed tissues Other technique, please specify ……………………………………………………………......…………………………… ……………………………………………………………......…………………………… 2. Are you working with: Isolated cells Other …………............................. Subcellular fractions 3. Is your protein post-translationally modified? Yes No Not known If yes, please indicate the amino acid number and the corresponding type of modification: ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… 4. Are you working under denaturing conditions? LIEGE Science Park • 4102 Seraing • BELGIUM RPM Liège • VAT (BE) - 0427.348.346 Tel.: +32 4 372 76 65 • Fax: +32 4 264 07 88 City: Yes No Not known 6. Have you already tried an immunization experiment for this protein? Yes No If yes, which peptides/protein sequences were used ? ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… In which type of experiments was the antibody used? ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… What were the results ? ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… 7. Remarks: ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… No Fax the completed order form to + 32 4 264 07 88 LIEGE Science Park • 4102 Seraing • BELGIUM • Tel.: + 32 4 372 76 65 • Fax: + 32 4 264 07 88 RPM Liège • VAT (BE) - 0427.348.346 • [email protected] • [email protected] • www.eurogentec.com > First-Class Program Evaluation Form The First Class Program Your purchase order reference: EGT Quotation Number: Antibodies that work in your application, guaranteed > Custom peptide antibodies adapted to VAT Nr. : If VAT exempt please include a copy of certificate DELIVERY ADDRESS INVOICE ADDRESS (Please fill in delivery information if different from invoicing information) Institute/Company: Institute/Company: Department/Lab.: Department/Lab.: Contact Person: Contact Person: Address: Address: your application > B-Epitopes are selected based on the antigen’s predicted 3D structural Postal Code: features in your application conditions Country: Country: Phone: Phone: Fax: Fax: e-mail: e-mail: > The right antibody for your immunoassay or your money back We have improved antigenic sequence prediction algorithms The antigenic surface of a protein is a 3-D patchwork of small linear antigenic sequences. Individually, each sequence is antigenic but, depending on the number of accessible residues in the interaction, the affinity will be either acceptable or too low. Currently, antibody affinities of 10-8 to 10-9 M can be expected for linear epitope, by calculating and analyzing the structure of each potential epitope. We will propose the most appropriate antigenic fragments that should exhibit such affinities. Ref: PRO-FIRSTCLASS-0207-V2 An epitope for each application As the structure of your protein may vary with each assay, an assay–antigen specific analysis must be made to determine structural and interaction properties. Major factors leading to changes in the epitope structure are (1) denaturation by detergent and (2) chemical modification of the amino acids of the epitope, for example with fixatives or other chemicals. For your immuno-assay technique the most exposed epitope may not be your best choice. Depending on whether the antibody will be used on a native, a detergent-denatured or a fixative-modified structure of your protein, we shall select either a flexible or a more rigid region of the protein such as a turn or a helix. Increased flexibility is reported to lead to improved affinity, however, rigid structures can provide good epitopes more resistant to detergent denaturation. Additionally, sequences containing aromatic residues rather than highly polar amino acids may be selected if application conditions will involve the use of chemicals that react with polar moieties. Indeed, as long as they do not impair the fragment accessibility, hydrophobic residues could improve the affinity. The prediction of the best epitope is closely linked to the application for which the antibody will be used. The “First Class” program – what do we do? Using a consensus of epitope prediction procedures we characterize all potential linear epitopes. Then, in a second step, we calculate their structures and keep those whose characteristics are adequate to raise high affinity antibodies. In the third step, we select the fragment(s) that are the most likely to be useful in your immuno-assay. What do we need ? The accession number of the protein of interest and a complete description of the application in which you will use the antibody. Please complete the questionnaire on the reverse side. We include • • • • • • • • • • Application specific peptide design 5 pre-immune rabbit sera for animal selection Synthesis of 2 peptides, 20-25 mg each Coupling of each peptide to a carrier protein Double X protocol in a 4-month program ELISA testing to monitor titer evolution Affinity purification of 5 ml of serum against each peptide Delivery of 15 - 20 mg of free peptide Remaining antisera All shipping costs City: Postal Code: Protein accession #: 1. For which experimental method do you want a guarantee? (only one technique please) [email protected] • [email protected] • www.eurogentec.com 5. Is your protein a membrane protein Yes ELISA in the absence of detergent or fixative Western Blot Immunoprecipitation with no detergent Immunoprecipitation in the presence of detergent Specify the concentration and the name of the detergent ………………………………………………………………...........…………………… Staining of chemically fixed tissues Specify the fixative ……….....................................……………...…… Staining of frozen-fixed tissues Other technique, please specify ……………………………………………………………......…………………………… ……………………………………………………………......…………………………… 2. Are you working with: Isolated cells Other …………............................. Subcellular fractions 3. Is your protein post-translationally modified? Yes No Not known If yes, please indicate the amino acid number and the corresponding type of modification: ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… 4. Are you working under denaturing conditions? LIEGE Science Park • 4102 Seraing • BELGIUM RPM Liège • VAT (BE) - 0427.348.346 Tel.: +32 4 372 76 65 • Fax: +32 4 264 07 88 City: Yes No Not known 6. Have you already tried an immunization experiment for this protein? Yes No If yes, which peptides/protein sequences were used ? ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… In which type of experiments was the antibody used? ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… What were the results ? ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… 7. Remarks: ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… ……………..…………………………………………………......…………………………… No Fax the completed order form to + 32 4 264 07 88 LIEGE Science Park • 4102 Seraing • BELGIUM • Tel.: + 32 4 372 76 65 • Fax: + 32 4 264 07 88 RPM Liège • VAT (BE) - 0427.348.346 • [email protected] • [email protected] • www.eurogentec.com
