A Covalently Linked 10 nm Gold Immunoprobe

Edmund Gutierrez, Richard D. Powell, James F. Hainfeld,* and Peter M. Takvorian**

Nanoprobes, Incorporated, Stony Brook, NY 11790.
* Biology Department, Brookhaven National Laboratory, Upton, NY 11973
** Biological Sciences Department, Rutgers University, Newark, NJ 07102.

We have prepared chemically functionalized, covalently linked 10 nm gold particles, which were conjugated to antibody Fab' fragments to yield highly effective imunogold probes, and may be cross-linked to other probes. 10 nm colloidal gold particles, prepared by the citrate reduction method,8 were stirred with a 10 : 1 mixture of two types of thioalkyl ligands, one functionalized with a solubilizing polyethylene glycol endcap moiety, the other with a protected amino-group. The stabilized nanoparticles were size separated by gel filtration (Superose-6, Pharmacia), deprotected by incubating at 50°C for 1 hour in 0.3N HCl / 20-40% alcohol, and converted to a maleimide derivative with sulfo-succinimidyl 4-[N-maleimido-methyl]cyclohexane-1-carboxylate (Sulfo-SMCC, Pierce). F(ab')₂ goat anti-mouse IgG or goat anti-rabbit IgG fragments were reductively cleaved to Fab' fragments using mercaptoethylamine hydrochloride (MEA) which selectively reduces the hinge disulfide bonds to give F(ab')₂ fragments, with 5 mm EDTA to prevent reoxidation. Fab' fragments were isolated by gel filtration over a coarse gel (GH25, Amicon) then mixed with the maleimido-gold particles. Conjugates were isolated by gel filtration (Superose-6, Pharmacia).

The Fab' goat anti-rabbit conjugate was used as a secondary probe to label a 43 kDa polar tube protein in spores of the microsporida Glugea americanus, a protozoan parasite which infects the nerves of the American Angler fish, Lophious americanus. The polar tube is a unique apparatus through which infective sporoplasm is transferred to host cells; its identification is diagnostic for microsporida, a class of organisms which are oportunistic in AIDS patients. Fixed G. americanus spores were dehydrated and embedded in LR White resin; thin sections were collected on nickel grids, dried and incubated overnight in a PBS/albumin blocking buffer containing normal goat serum. Grids were incubated for two hours with monoclonal anti-PTP 43 GA antibody, followed by 10 nm gold-Fab' anti-mouse or 12 nm gold-IgG anti-mouse (Jackson) secondary and stained with uranyl acetate. The polar tube was labeled clearly. In immunoblotting experiments against serial dilutions of mouse IgG spotted onto a nitrocellulose membrane, the covalently linked probe showed the same sensitivity as a conventional 10 nm colloidal gold conjugate; however, background staining was significantly lower (Figure 4). Control experiments were conducted in which the conjugation procedure was repeated (a) without converting the gold to maleimide, or (b) without reducing the F(ab')₂. In both cases, immunoblot sensitivities were reduced by factors of more than 10, showing that covalent linking is necessary for full probe activity.

References

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8. Ths work was partly supported by SBIR grant number R44 GM50048.

FIGURES 1-3: Electron micrographs of G. americanus spores incubated with monoclonal anti-PTP 43 GA primary antibody with (1) 12 nm colloidal gold anti-mouse secondary (Jackson), and (2) and (3) 10 nm covalent gold-Fab' anti-mouse. Polar tube labeling shown by arrows (bar = 0.5 micrometer).

FIGURE 4: Immunoblot of 10 nm colloidal gold-IgG (A) and 10 nm covalent gold-Fab' (B) anti-mouse conjugate against serial dilutions of mouse IgG spotted onto nitrocellulose membrane; (C) key showing the amounts of mouse IgG in each spot for the corresponding divisions of the blots.

Other Applications:

Product Applications Special report: A very reliable pre-embedding immunogold method. Our 2002 paper: Nickel-NTA-Nanogold Binds his-Tagged Proteins. Our 2001 paper on DNA Nanowires. Our 1999 paper on Gold-Based Autometallography. Special report: In Situ Hybridization with Nanogold®-Streptavidin. Technical note: Nanogold® Staining on Gels. Our 1996 paper on Gold Liposomes. Special report: Nanogold® Labeling of Peptides. Technical note: RNA Labeling with Nanogold®. Our 1991 paper on A New 1.4 nm Gold-Fab' Probe. Our 1994 paper on Methylamine Vanadate (NanoVan) Negative Stain. Our 1990 paper on Conducting Polymer Films as EM Substrates. Research Applications Our 2005 paper: 5 nm Gold-Ni-NTA binds His Tags. Enzymatic Metallography: A Simple New Staining Method Our 2006 paper on Light and Electron Microscopy of Microsporida using Enzyme Metallography. Our 2004 paper on Enzymatic Metallography as a Correlative Light and Electron Microscopic Method. Our 2002 paper on Enzymatic Metallography: A Simple New Staining Method.

Research Applications (continued) Our 2007 paper on Correlative Enzymatic and Gold Probes for Light and Electron Microscopy. Our 1995 paper on Aldehyde Gold Clusters for Molecular Labeling. Our 2000 paper on Gold Cluster Crystals. Larger covalent gold probes: Our 2005 paper on Preparation of Covalent 3nm Gold – Fab’ Probes. Our 1999 paper on A Covalently Linked 10 nm Gold Immunoprobe. Combined fluorescent and gold probes: Our 2003 paper featuring Dextran-Texas Red®-Nanogold® Fluorescent Dyes for Use in Correlative Microscopy and Intravital Imaging. Our 2002 paper on Combined ALEXA-488 and Nanogold Antibody Probes. Our 1999 paper on Combined Cy3 / Nanogold Probes for Immunocytochemistry and In Situ Hybridization. Our 1998 paper on Dual-Labeled Probes for Fluorescence and Electron Microscopy. News: our original 1997 paper on Combined Fluorescent and Gold Immunoprobes. Our 1996 paper on Large Cluster and Combined Fluorescent and Gold Immunoprobes. Our 1994 paper on Combined Fluorescent and Gold Nucleic Acid Probes. Our 2005 paper on High Z Metal Carbonyls for Imaging and Microspectroscopy. Our 2005 paper on In Vivo Vascular Casting.