carbocyanines and isothiocyanic-acid

carbocyanines has been researched along with isothiocyanic-acid* in 2 studies

Other Studies

2 other study(ies) available for carbocyanines and isothiocyanic-acid

Article	Year
Spherical vs. granular immobilization support selection and performance on an optical flow cell immunosensor based on the fluorescence of Cyanine-5. Preparative biochemistry & biotechnology, 2006, Volume: 36, Issue:4 A spherical porous glass support Trisoperl (TRISO) with four pore diameters (ø 47.8; 55.9; 102.6, and 108.8 nm) was characterized and selected for application in an optical flow cell immunosensor, in comparison with controlled pore glass (CPG). The TRISO support was functionalized with aldehyde and isothiocyanate (-NCS) groups to attach bovine serum albumin and alkaline phosphatase (AP). The TRISO isothiocyanate pore diameter 47.8 nm (TRISO(-NCS) 47.8 nm) showed the better potential to be used in the immunosensor. It immobilized more protein (19.3 mg AP per g support) while presenting an optical performance comparable to the CPG. CPG(-NCS) and TRISO(-NCS) 47.8 nm were tested in the immunosensor model where the saturation of the Goat IgG immobilized in the supports with Monoclonal Anti-Goat IgG conjugated with Cyanine-5 was reached, followed by regeneration with the elution buffer modified PBS pH 2.0. The TRISO(-NCS) 47.8 nm presented lower fluorescence intensity at saturation (around 39 AU) than CPG(-NCS) (150 to 104 AU), but revealed a major advantage related to the uniform arrangement of the spherical particles in the flow cell, generating no significant fluorescence differences between gravity and flow package. Topics: Aldehydes; Alkaline Phosphatase; Animals; Antibodies, Monoclonal; Biosensing Techniques; Carbocyanines; Cattle; Enzymes, Immobilized; Fluorescent Dyes; Glass; Immunoglobulin G; Isothiocyanates; Optics and Photonics; Serum Albumin, Bovine; Surface Properties	2006
Cyanine dye labeling reagents containing isothiocyanate groups. Cytometry, 1989, Volume: 10, Issue:1 New isothiocyanate derivatives of cyanine dyes were synthesized as fluorescent covalent labeling reagents for proteins and other biomolecules. These dyes have maximum absorbance in the red and near infrared regions of the spectrum, have high extinction coefficients and have adequate quantum yields. Incorporating two alkyl sulfonate groups in the dye structures increases their water solubility, which is beneficial for labeling biological molecules in aqueous solution. Reactivities of proteins with these new cyanines are similar to their reactivities with fluorescein isothiocyanate. These new labeling reagents are complementary to the fluorescein and rhodamine reagents, expanding the possibilities of multicolor analyses. Sheep anti-mouse-IgG antibody was labeled with a pentamethine cyanine dye (CY5.8-ITC) and used with a fluoresceinated antibody as a second reagent for detecting human T-cell subsets by flow cytometry. Topics: Antibodies; Carbocyanines; Flow Cytometry; Fluorescent Dyes; Humans; Immunoglobulins; Indicators and Reagents; Isothiocyanates; Lymphocytes; Proteins; Quinolines; Spectrometry, Fluorescence; Terminology as Topic; Thiocyanates	1989

Article

Year

Spherical vs. granular immobilization support selection and performance on an optical flow cell immunosensor based on the fluorescence of Cyanine-5.

Preparative biochemistry & biotechnology, 2006, Volume: 36, Issue:4

A spherical porous glass support Trisoperl (TRISO) with four pore diameters (ø 47.8; 55.9; 102.6, and 108.8 nm) was characterized and selected for application in an optical flow cell immunosensor, in comparison with controlled pore glass (CPG). The TRISO support was functionalized with aldehyde and isothiocyanate (-NCS) groups to attach bovine serum albumin and alkaline phosphatase (AP). The TRISO isothiocyanate pore diameter 47.8 nm (TRISO(-NCS) 47.8 nm) showed the better potential to be used in the immunosensor. It immobilized more protein (19.3 mg AP per g support) while presenting an optical performance comparable to the CPG. CPG(-NCS) and TRISO(-NCS) 47.8 nm were tested in the immunosensor model where the saturation of the Goat IgG immobilized in the supports with Monoclonal Anti-Goat IgG conjugated with Cyanine-5 was reached, followed by regeneration with the elution buffer modified PBS pH 2.0. The TRISO(-NCS) 47.8 nm presented lower fluorescence intensity at saturation (around 39 AU) than CPG(-NCS) (150 to 104 AU), but revealed a major advantage related to the uniform arrangement of the spherical particles in the flow cell, generating no significant fluorescence differences between gravity and flow package.

Topics: Aldehydes; Alkaline Phosphatase; Animals; Antibodies, Monoclonal; Biosensing Techniques; Carbocyanines; Cattle; Enzymes, Immobilized; Fluorescent Dyes; Glass; Immunoglobulin G; Isothiocyanates; Optics and Photonics; Serum Albumin, Bovine; Surface Properties

2006

Cyanine dye labeling reagents containing isothiocyanate groups.

Cytometry, 1989, Volume: 10, Issue:1

New isothiocyanate derivatives of cyanine dyes were synthesized as fluorescent covalent labeling reagents for proteins and other biomolecules. These dyes have maximum absorbance in the red and near infrared regions of the spectrum, have high extinction coefficients and have adequate quantum yields. Incorporating two alkyl sulfonate groups in the dye structures increases their water solubility, which is beneficial for labeling biological molecules in aqueous solution. Reactivities of proteins with these new cyanines are similar to their reactivities with fluorescein isothiocyanate. These new labeling reagents are complementary to the fluorescein and rhodamine reagents, expanding the possibilities of multicolor analyses. Sheep anti-mouse-IgG antibody was labeled with a pentamethine cyanine dye (CY5.8-ITC) and used with a fluoresceinated antibody as a second reagent for detecting human T-cell subsets by flow cytometry.

Topics: Antibodies; Carbocyanines; Flow Cytometry; Fluorescent Dyes; Humans; Immunoglobulins; Indicators and Reagents; Isothiocyanates; Lymphocytes; Proteins; Quinolines; Spectrometry, Fluorescence; Terminology as Topic; Thiocyanates

1989