Combined ALEXA-488 and Nanogold Antibody Probes

W. Liu, J. F. Hainfeld, and R. D. Powell

Nanoprobes, Incorporated, 95 Horseblock Road, Yaphank, NY 11980

A combined ALEXA 488 and Nanogold probe was prepared by the reduction of F(ab’)2 Goat anti-Mouse IgG to Fab’ fragments with mercaptoethylamine hydrochloride (MEA), which selectively reduce the F(ab’)2 hinge disulfide bonds, with 5 mm EDTA present to prevent reoxidation. Fab’ fragments were isolated by gel filtration (coarse gel: GH25, Millipore) then labeled selectively at the reduced hinge thiol using Monomaleimido-Nanogold [5]. The conjugate was isolated by gel filtration (Superose-12, Pharmacia), then reacted with excess ALEXA Fluor 488 amine labeling kit (Molecular Probes); dual-labeled conjugates were isolated by gel filtration (Superose-12). In this way, the fluorescent group was positioned sufficiently far from the Nanogold that quenching through fluorescence resonance energy transfer [1] was minimized. UV/visible spectroscopy indicated incorporation of 2-3 ALEXA molecules per Fab’; preliminary fluorescence measurements suggested that fluorescence emission intensities relative to the unconjugated ALEXA dye were more than twice those of combined fluorescein and Nanogold conjugates relative to unconjugated fluorescein.

The combined ALEXA 488 and Nanogold conjugate was used to stain cytokeratin in paraffin-embedded human prostate carcinoma test slides; bright, clear fluorescence labeling was found, as shown in Figures 1 and 2. Localization of the gold was demonstrated by brightfield microscopy after silver enhancement (Figure 3); specificity was confirmed by the absence of labeling when the primary antibody was omitted (Figure 4). Further experiments are in progress to characterize and optimize the performance of this probe, and to prepare combined fluorescent and Nanogold probes using other ALEXA dyes.

References

1. R. D. Powell, C. M. R. Halsey, and J. F. Hainfeld: Microsc. Res. Tech., 42 (1998) 2.

2. T. Takizawa, K. Suzuki, and J. M. Robinson: J. Histochem. Cytochem., 46 (1998) 1097.

3. R. D. Powell, V. N. Joshi, C. M. R. Halsey, J. F. Hainfeld, G. W. Hacker, C. Hauser-Kronberger, W. H. Muss, and P. M. Takvorian,: Microsc. Microanal., (Suppl. 2: Proceedings), 6 (1999) 478.

4. N. Panchuk-Voloshina, R. P. Haugland, J. Bishop-Stewart, M. K. Bhalgat, P. J. Millard, F. Mao, and W. Y. Leung: J. Histochem. Cytochem., 47 (1999) 1179.

5. J. F. Hainfeld and F. R. Furuya: J. Histochem. Cytochem., 40 (1992) 177.

6. The authors thank Molecular Probes for providing ALEXA Fluor 488 amine labeling reagent. This project was partly supported by SBIR grant 1R43 GM62100-01 from the National Institute of General Medical Sciences (National Institutes of Health).

Figure 1: Fluorescence micrograph of paraffin section of human prostate carcinoma (Dako Cytokeratins Human Adeno CA prostate slide) stained for cytokeratin using monoclonal primary antibody (AE1/AE3, Dako: 1 : 50 dilution in Tris-buffered saline), and combined ALEXA-488/Nanogold-Fab’ goat anti-Mouse IgG (final concentration 28 mg/mL) secondary (bar = 100 microns).

Figure 2: Higher magnification view of same specimen as Figure 1 (bar = 25 microns).

Figure 3: Brightfield light micrograph of paraffin section of human prostate carcinoma (Dako Cytokeratins Human Adeno CA prostate slide) stained for cytokeratin as in Figure 1, followed by silver enhancement with LI Silver (Nanoprobes) for 15 minutes (bar = 25 microns).

Figure 4: Negative control: paraffin section of human prostate carcinoma (Dako Cytokeratins Human Adeno CA prostate slide) stained and silver enhanced as in Figure 3, except that primary antibody was omitted (bar = 25 microns).

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.