The RT-PCR products were resolved on 2% (wt/vol) agarose gel and stained by GoldView (Beijing SBS Genetech Co) (Figure S1C).

The human CD147 mutants (K234R, K250R, K259R, and K261R) were generated from the eGFP-N1-CD147 plasmid using a site-directed mutagenesis kit (SBS).

HPLC purified oligonucleotides were procured from SBS Genetech, China.

The formed digestion products were separated on 4% agarose gels and stained with GoldView (SBS Genetech Beijing, China).

Single-cell suspensions were pulsed with 1 μM hgp100_25–23 (KVPRNQDWL) of immunograde quality, which was purchased from SBS (Beijing SBS Genetech Co. Ltd., Beijing, China).

The restriction products were electrophoresed on a 3% agarose gel, and visualized by staining with Gold View (SBS Genetech).

The FITC-labeled control aptamer NK8 (bound to Mycobacterium tuberculosis) was synthesized by SBS Genetech Co., Ltd.

Total RNA from S. gilvosporeus strains was prepared with Redzol reagent and extracted using the Total RNA extraction kit (SBS Genetech Co., Ltd.), according to the manufacturer's instructions.

Single point mutants of TRPV1 were obtained by using Fast Mutagenesis Kit V2, (SBS Genetech Co.,Ltd., China) which were sequenced to confirm that site-directed mutagenesis was made.

Human pIgR mutants were generated using the Muta-direct Site-directed Mutagenesis kit (Beijing SBS Genetech Co, Ltd, Beijing, China).