From a literature search performed up to December 2017, we retrieved 12 missense HTRA1 alleles identified in symptomatic carriers: S121R, A123S, R133G, R166C, R166L, A173P, S284G, S284R, P285Q, F286V, G295R, and D450H; and 3 missense HTRA1 alleles reported only in CARASIL patients: A173T, A321T, and L364P (5, 8–12). Clinical characteristics of the symptomatic carriers are summarized in Supplemental Table 1. This study was approved by the Niigata University institutional review board.

An expression plasmid for each variant HTRA1 cDNA was generated using the GENEART® Site-Directed Mutagenesis System (Invitrogen, Carlsbad, CA). The WT-HTRA1 cDNA tagged with a C-terminal myc-His₆ was subcloned into the pcDNA 3.1 vector (Invitrogen) was the substrate for mutagenesis. The concentration of each plasmid was measured using the Quant-iT^TM PicoGreen dsDNA Assay Kit (Thermo Fisher Scientific, Waltham, MA, USA). The HTRA1 cDNA plasmid vectors were transfected into FreeStyle 293 cells (Thermo Fisher Scientific) and incubated for 72 h. After incubation, secreted HTRA1 protein was purified from the culture medium using a HisTrap FF crude column (GE Healthcare, Cleveland, OH, USA). The concentration of recombinant HTRA1 proteins was measured using a Bicinchoninic Acid (BCA) Protein Assay Kit (Wako, Osaka, Japan). After pre-incubating 1 μg of the recombinant HTRA1 protein, protease activities were evaluated at 37°C using fluorescein isothiocyanate (FITC)–labeled casein as a substrate (Fluorescent Protease Assay Kit; Pierce, Rockford, IL, USA) (2, 6). WT was used as the positive control and S328A, which is deficient in protease activity, was used as the negative control. Fluorescence was measured using a FilterMax F5 Multi-Mode Microplate Reader (Molecular Devices, Sunnyvale, CA, USA). Protease activities were calculated from the slope of the linear portion of the normalized fluorescence vs. time plots at 30, 60, and 90 min using MATLAB® R2017b (9.3.0.713579). The amount of each HTRA1 protein was analyzed by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE), stained by SYPRO® Ruby Protein Gel Stain (Thermo Fisher Scientific). Five mutations, S121R, A123S, R133G, S284G, and D450H, were excluded from further analysis because the protease activities of these mutations were normal (Figure 1B); two of these five mutations were appeared to be benign (A123S and R133G) (5).

Oligomerization was evaluated by size-exclusion chromatography using a Superdex 200 10/300 GL column (GE Healthcare, Chicago, IL, USA) on an AKTA FPLC workstation equilibrated with Tris-buffered saline (100 mM Tris-HCl, pH 8.0 and 150 mM NaCl). After pre-incubation at 37°C for 30 min, each HTRA1 protein sample was injected at 500 ng/μl. Y169E/F171E HTRA1, an artificial, known monomeric HTRA1, was used as the reference monomer and S328A HTRA1 was used as a reference trimer (Figure 2C) (4, 6). SDS-PAGE was used to evaluate fractions from size-exclusion chromatography (6).

Each HTRA1 variant vector was cotransfected with an equal amount of WT vector into FreeStyle 293 cells. Purification of the mixed HTRA1 proteins and evaluation of their protease activity were performed as described above. We compared the protease activities of the mixtures of WT with each variant HTRA1 to that of a mixture of WT and S328A, an artificially inactive HTRA1 that forms a trimer with WT and does not have a dominant-negative effect; this was used as a reference to adjust the protein concentration in the reaction mixture (6). The mixtures of G283E with WT and A252T with WT were used as positive and negative controls for dominant-negative effects, respectively (6).

Statistical analyses were performed using R 3.2.2. Groups were compared using one-way analysis of variance (ANOVA) for independent samples, followed by Dunnett's multiple-comparison test when overall P was < 0.05. Fisher's exact test was used to compare the frequencies of mutant HTRA1s with dominant-negative effect between symptomatic carriers and CARASIL.

Five missense HTRA1s (S121R, A123S, R133G, S284G, and D450H) showed normal protease activity, thus we excluded these HTRA1s from further analysis (Figures 1A,B). Protease activities of other HTRA1s were significantly decreased relative to WT activity. We assayed trimerization of the other HTRA1s and found that four hetero-HTRA1s (R166C, R166L, A173P, and G295R) and one CARASIL-HTRA1 (A173T) were unable to form trimers (Figures 2A,B). Among mutant HTRA1s form trimers, all hetero-HTRA1s had mutations in the LD domain (residues 284–290) or L3 loop domain, (residues 301–314) while two CARASIL-HTRA1s had mutations in the protease domain (residues 204–356) (Table 1).

Next we investigated whether these missense HTRA1s have dominant-negative. To serve as a control for this assay, the half dose of WT was not suitable because protein and substrate concentrations in the reaction mixture differ from those expressing WT and each mutant HTRA1 (6). Therefore, we used a mixture of WT and S328A, an artificial inactive HTRA1 that trimerizes, as a control (3, 4) and compared the protease activities of the mixtures of WT and each mutant HTRA1 with that of the control. dominant-negative was then defined as a protease activity less than that of the control. Four of six hetero-HTRA1s and one of four CARASIL-HTRA1 showed dominant-negative (Figure 3 and Supplemental Figure 1).

The results showed the possibility that the HTRA1 mutant proteins identified in the symptomatic carriers cannot form trimers or have mutations in the LD or L3 domain. Therefore, we examined the frequency of mutant HTRA1s with these characteristics between missense mutations identified in symptomatic carriers and only in CARASIL. Combined with our previous results, all missense HTRA1s identified in symptomatic carriers were defective in trimerization or had mutations in the LD or L3 domain, but only two of six missense HTRA1s found only in CARASIL patients were defective in trimerization and none had mutations in the LD or L3 domain (P = 0.006; Table 1). In contrast, the frequency of mutant HTRA1s with dominant-negative effects in symptomatic carriers was not significantly higher than that in CARASIL patients (72.7 vs. 33.3%, P = 0.162; Table 1).

OO has received speaking honoraria from Kyowa Hakko Kirin Co., Ltd., Bristol-Myers Squibb, Ono Pharmaceutical Co., Ltd., Mitsubishi Tanabe Pharm, Takeda, Daiichi-Sankyo, FUJIFILM, SANOFI, and FP-pharm. The remaining authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.