This journal is (c) The Royal Society of Chemistry 21 Zeta potential based Colorimetric Immunoassay for the direct detection of Diabetic marker HbA1c using Gold Nanoprobes Nishima Wangoo, a,b Jyotsna Kaushal, c K.K.Bhasin, b S.K.Mehta b and C Raman Suri* a a Institute of Microbial Technology (CSIR), Sector 39-A, Chandigarh 1614, India b Chitkara Institute of Engineering &Technology, Rajpura, Distt. Patiala, India c Department of Chemistry and Centre of Advanced Studies in Chemistry, Panjab University, Chandigarh 1614, India Supporting Information Experimental Procedure
This journal is (c) The Royal Society of Chemistry 21 Generation and Purification of anti HbA1c antibodies Anti-HbA1c antibodies were raised by immunizing young white New Zealand rabbits using standard immunization protocol (Fig. S1). Rabbits were immunized with 3 μg of each serum proteins (HbA1c) emulsified in CFA for first injection and in IFA for booster doses which were repeated 3-4 times every 21 days and sera were collected on th day after each booster. After de-complementation at 6 C for 3 minutes, it was stored in aliquots at - 2 C. The sera were pooled and precipitated under constant stirring at 4 C at % saturated ammonium sulfate and centrifuged. The precipitate was dissolved in minimum volume of PBS and was extensively dialyzed against PBS (ph 8.) at 4 C. It was then passed through the protein-a sepharose column and bound antibody was eluted with.1m glycine-hcl buffer (ph 2.). Fractions were neutralized immediately with 1M Tris (ph 8.) and dialyzed extensively against PBS ph 7.4 at 4 C, and stored in aliquots at 2 C. Concentration was determined by taking absorbance at 28 nm and by taking 1.3 as extinction coefficient. Critical Flocculation Concentration Assay and Synthesis of Antibody-GNP conjugate In this assay, 1 μl of antibody solution prepared at different concentrations in phosphate buffer (2mM, ph 7.4) was added to tubes containing 1 ml of the colloidal gold solution. After 1 min, flocculation was induced by adding 1 μl of 1% NaCl and absorbance was measured at 8 nm. The amount of protein necessary to prevent flocculation was deduced graphically from the concentration at which the absorbance becomes nearly constant. For preparing Ab-GNPs conjugates, anti-hba1c antibodies prepared in phosphate buffer were added separately into 1 ml colloidal gold solution under mild stirring conditions. The ph of the colloidal gold solution was maintained at 7.4 by addition of dilute.1m K 2 CO 3 before adding the antibody concentration derived from CFC measurements. The mixture was incubated overnight at 4 C and centrifuged at 12, rpm for 3 min. The pellet obtained was further washed twice with 1 mm Tris (ph 8.) under centrifugation at 12, rpm for 3 min to remove traces of unconjugated antibody. Nanoprobe based Immunoassay The homogeneous immunoassay was conducted in solution using the antibodyconjugated nanoparticles ( µl) into each well of micro titre strip (Nunc, USA). Serial
This journal is (c) The Royal Society of Chemistry 21 dilutions of the antigen were prepared in carbonate buffer and µl of sample was added to each well followed by the addition of µl of NaCl (M) after min. The absorbance at 2 nm and 62 nm were measured using an ELISA plate reader (Biotech, USA). All experiments were performed at room temperature.
This journal is (c) The Royal Society of Chemistry 21 Figures for ESI.2 Absorbance (a.u.).18.16.14.12.1.8.6 a b c (a-2 nm) (b-4 nm) (c-7 nm).4 4 4 6 6 Wavelength (nm) Figure S1: UV Vis spectra recorded from the colloidal gold solutions reduced with glutamic acid of different concentrations. Inset shows the corresponding TEM images of the GNPs solutions. Scale bar =1 nm. 3. 3. BSA OVA HSA GHb Mean OD at 4 nm 2. 2. 1. 1... 1 2 3 Booster Dose Figure S2: Binding of anti-hba1c antibody with BSA (Bovine Serum Albumin), OVA (Ovalbumin), HSA (Human serum albumin) and GHb (Glycated Haemoglobin)
Supplementary Material (ESI) for Chemical Communications This journal is (c) The Royal Society of Chemistry 21 Zeta Potential Measurements 1 4 4 2 1 8 2-8 -13.2mV -2 2 1 1-2 (g) 1 (f) -8.34mV -1.82mV -2 (e) (d) 2 1 1-8 (c) -17.34mV -19.2 mv (b) 8 3 2-4 (a) 3 1-4 -24.2 mv -28.9 mv 1 2 1-39 mv 1 3.44mV 1 2 (h) -2 4-4 (i) Figure S4: Zeta potential measurements for (a) GNP, (b) GNP-Ab, (c)-(i) variation in zeta potential of 4 nm GNPs aggregates with increasing amount of the antigen HbA1c.
Supplementary Material (ESI) for Chemical Communications This journal is (c) The Royal Society of Chemistry 21 4.8 23.1 11.8 43.9 nm 1. 16 31 187.4 Differential (%) Differential (%) 7 nm 32.7 6 nm 1 1 23.6 11 nm 37.4 228.6 13 Differential (%) Differential (%) 2.3 127.3 6.7 131. 99 nm 1. 3.9 34.4 21.4 111 (f) (e) (g). (d) 6.1 1. (c) 1. 4.6 nm (b).7 9 (a) 1. 173. Differential (%) 1. Differential (%) 4 nm 216 nm Differential (%) Differential (%) Differential (%) Dynamic (DLS) measurements 38 nm c 1. 8.1 6.1 2.4 39 (h) 2. 7.4 164.7 472.6 (i) Figure S: DLS measurements for (a) GNP, (b) GNP-Ab, (c)-(i) variation in size of 4 nm GNPs aggregates with increasing amount of the antigen (HbA1c). 13