Tao Y , Aparicio T , Li M , Leong KW , Zha S , Gautier J .

R35 CA197606 NCI NIH HHS , R50 CA233182 NCI NIH HHS , P01 CA174653 NCI NIH HHS , R01 CA158073 NCI NIH HHS , R01 CA215067 NCI NIH HHS

             DNA damage checkpoint
             DNA replication
             DNA repair
             nucleosome assembly
             nuclear membrane

	Figure 1. Synthesis and characterization of silver nanoclusters (AgNCs). (A) Schematic diagram of AgNCs. (B) Absorbance and fluorescence spectra of AgNCs. (C) Transmission electron microscopy (TEM) image and corresponding size distribution histogram of AgNCs. Scale bars, 20 nm. (D) Zeta potential and hydrodynamic diameter of AgNCs.
	Figure 2. AgNCs uniquely inhibit DNA replication and replication checkpoint. (A, B) DNA replication in extracts is sensitive to AgNCs. (A) Xenopus egg extracts were incubated with sperm nuclei in the presence of increasing concentrations of AgNCs. DNA replication was monitored by agarose gel electrophoresis after incorporation of α-[32P]dCTP into genomic DNA. (B) Quantification of three independent experiments normalized to untreated controls. (C, D) AgNCs inhibit the DNA replication checkpoint. (C) Xenopus egg extracts were treated with aphidicolin with or without AgNCs at different concentrations and incubated with sperm nuclei. ATR activation was monitored by pChk1 western blotting. (D) Quantification of three independent experiments normalized to aphidicolin alone control. Impact of different silver nanomaterials on DNA replication and replication checkpoint. (E) Replicating extracts were incubated with silver ions (Ag+), silver nanoparticles (AgNPs), silver nanoprisms (AgNPrs) and silver nanoclusters (AgNCs) and DNA replication was assessed by incorporation of α-[32P]dCTP into genomic DNA. (F, G) The impact of Ag+, AgNPs, AgNPrs AgNCs and PAA on DNA replication checkpoint was monitored by pChk1 Western blotting.
	Figure 3. AgNCs affect DNA replication initiation. (A, B) Time-course of DNA replication assay. (A) Experiment time-course showing the time of AgNCs addition to DNA replication assay. (B) AgNCs were added to extracts at different time points during DNA replication (T = –10, 0, 20, 40, 60 min) and DNA replication products were monitored by agarose gel electrophoresis at 80 min after addition of AgNCs. For the first lane (control), no AgNCs were added and replication was monitored at 80 min. (C, D) AgNCs block pre-RC assembly. (C) Chromatin binding assays were performed in Xenopus egg extracts supplemented with demembranated sperm nuclei (2500 sperm/μl) and incubated for 10 min at 21°C for chromatin assembly following addition of AgNCs at indicated timepoints (10, 30, 60 and 90 min). Chromatin was isolated through 30% sucrose cushions and bound proteins were resolved by SDS-PAGE on 10% Bis-Tris gels and probed with specific antibodies against MCM3, RPA and histone H3. (D) The mean and standard deviation is shown for three ieendependent biological replicates.
	Figure 4. AgNCs interact with MCM protein complex. (A) Synthesis of FLAG-AgNCs (FLAG peptide: CGGMDYKDHDADYKDHDIDYKDDDDK). The decrease of FLAG peptide absorbance in the filter indicated the successful linkage of FLAG peptide on AgNCs. (B) FLAG-tagged AgNCs inhibits the DNA replication checkpoint. Xenopus egg extracts were treated with aphidicolin with or without AgNCs or FLAG-AgNCs and incubated with sperm nuclei. ATR activation was monitored by pChk1 western blotting. (C, D) Chromatin binding assay in the presence of FLAG-AgNCs. (C) Schematic representation of the experiments. (D) Chromatin was isolated through 30% sucrose cushion and bound proteins (ORC1, CDC6, MCM3, RPA and histone H3) resolved by 3%-8% gradient Tris-Acetate gels followed by western blot. Left: control, untreated extarcts. Right: extracts incubated with FLAG-tagged AgNCs. (E) Xenopus egg extracts were incubated with FLAG peptide (control) or FLAG-AgNCs, immunoprecipitated with anti-FLAG antibodies, whashed and processed for western blot with ORC1, CDC6 and MCM3 antibodies. (F) Xenopus egg extracts were incubated for 1 h with FLAG-AgNCs. Following FLAG immunoprecipitation, AgNCs-bound proteins were identified by mass spectrometry. MCM polypeptides recovered are indicated. (G) Purified hexameric MCM complex expressed in baculovirus-infected cells was incubated with FLAG-AgNCs in vitro. Bound and soluble fractions were processed for Western blotting with MCM3 antibodies.
	Figure S1. Synthesis and characterization of silver nanoparticles (AgNPs) and silver nanoprisms (AgNPrs). (a, d) Absorbance and fluorescence spectra of AgNPs and AgNPrs. (b, d) Transmission Electron Microscopy (TEM) images of AgNPs and AgNPrs. Scale bars, 50 nm. (c, f) Zeta potential and hydrodynamic diameter of AgNPs and AgNPrs. We confirmed the successful generation of silver nanoparticles (AgNPs) and silver nanoprisms (AgNPrs) by optical absorption and transmission electron microscopy (TEM). As shown in Figure S2a, AgNPs exhibit the characteristic absorption peaks at 420 nm, which are assigned to AgNPs (1,7). Figure S2b shows typical TEM image of the AgNPs prepared as described, in which AgNPs were monodispersed with an average size of about 10 nm. Dynamic light scattering characterization (Figure S2c) indicates that zeta potential and hydrodynamic diameter of AgNPs were –19.64 ± 1.34 mV and 13.44 ± 1.22 nm, respectively. Similarly, we also assessed the properties of the AgNPrs by monitoring the UV−vis absorption spectra, the size and shape by transmission electron microscopy (TEM) and the zeta potential. Figure S2d shows the UV−vis absorption spectrum of AgNPrs with two characteristic bands at 665 nm ascribed to in-plane dipole resonance and at 335 nm corresponding to out-of-plane quadrupolar resonance (2,8). The representative TEM picture in Figure S2e shows that AgNPrs exhibited a triangular prism structure with an edge length between 30 and 40 nm. Dynamic light scattering and zeta potential measurements (Figure S2f) indicate that the average hydrodynamic size and surface charge are about 43.27 nm and −14.51 mV, respectively.
	Figure S2. (a) Normalized fluorescence intensity of AgNCs after 6 hours incubation in water or in replication assay buffer. (b) Hydrodynamic diameter of AgNCs in water and in replication assay buffer.
	Figure S3. Replicating extracts were incubated with PAA and Ag ions in the presence of PAA for 90 minutes, and DNA replication was assessed by incorporation of α-[32P]dCTP into genomic DNA.
	Figure S4. (a) Replicating extracts were incubated with gold nanoclusters (AuNCs), copper nanoclusters (CuNCs), carbon dots (CDs) and silver nanoclusters (AgNCs) for 90 minutes, and DNA replication was assessed by incorporation of α-[32P]dCTP into genomic DNA. (b) The impact of AuNCs, CuNCs, CDs and AgNCs on DNA replication checkpoint was monitored by pChk1 Western blotting.
	Figure S5. AgNCs does not inhibit nuclear assembly. (a) Schematic representation of the experiments. (b) Nuclear assembly in Xenopus egg extracts in the presence of AgNCs. Nuclear formation was followed over the course of 45 min by fluorescence microscopy with DAPI.
	Figure S6. Micrococcal nuclease digestion of chromatin fractions in assembled in LSS extracts in the presence of AgNCs. Chromomal DNA was purified after nuclease digestion for the indicated times and separated by 1.5% TBE-agarose gel electrophoresis.
	Figure S7. AgNCs do not impact ORC and CDC6 chromatin recruitment. AgNCs were added to LSS extracts at 0, 20 or 40 minutes after sperm chromatin addition. Chromatin was isolated and probed by Western blotting with the indicated antibodies.
	Figure S8. Absorbance fluorescence spectrum of FLAG-AgNCs.

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