Identification of End-Binding 1 Protein as Novel α-4 Giardin-Binding Partners in Giardia lamblia Trophozoites

Background Giardia lamblia (syn. G. intestinalis, G. duodenalis) is a primitive opportunistic protozoon, and one of the earliest differentiated eukaryotes. Despite its primitive nature, G. lamblia has a sophisticated cytoskeleton system, which is closely related to its proliferation and pathogenicity. Meanwhile, α giardin is a G. lamblia-specific cytoskeleton protein, which belongs to the annexin superfamily. Interestingly, G. lamblia has 21 annexin-like α giardins, i.e., more than higher eukaryotes. The functional differences among α giardin members are not fully understood. Methods We took α-4 giardin, a member of α giardin family, as a research object. A morpholino-mediated knockdown experiment was performed to identify the effect of α-4 giardin on G. lamblia trophozoites biological traits. A yeast two-hybrid cDNA library of G. lamblia strain C2 trophozoites was screened for interaction partners of α-4 giardin. Co-immunoprecipitation and fluorescent colocalization confirmed the relationship between G. lamblia EB1 (gEB1) and α-4 giardin. Results α-4 Giardin could inhibit the proliferation and adhesion of G. lamblia trophozoites. In addition, it interacted with G. lamblia EB1 (gEB1). Conclusions α-4 Giardin was involved in proliferation and adhesion in G. lamblia trophozoites, and EB1, a crucial roles in mitosis, was an interacting partner of α-4 giardin.


Introduction
Giardia lamblia (syn.G. intestinalis, G. duodenalis), a common, opportunistic intestinal parasitic protozoa with worldwide distribution, can parasitize the small intestine of humans and many other mammals, causing giardiasis that mainly manifests as diarrhea, abdominal pain, nausea and malabsorption symptoms.The life cycle of G. lamblia includes the infective, immotile cyst and the vegetative, motile trophozoite.Cysts are resistant forms and responsible for the transmission of giardiasis.After cysts pass through the stomach, they are transformed into trophozoites.G. lamblia trophozoites attach strongly to intestinal epithelial cells via a ventral adhesive disc, a concave cytoskeletal structure surrounded by the plasma membrane, and cause significant damage and disruption to the intestinal epithelium [1,2].
As one of the earliest diverging eukaryotes, G. lamblia represents an excellent model system for assessing basic eukaryotic processes [3].G. lamblia is only a primitive eukaryotic unicellular organism which has a highly developed and fine cytoskeleton system similar to that of higher eukaryotes, but the structures formed by these proteins in G. lamblia are unique.Microtubules, microfilaments, and related proteins forming the cytoskeleton mainly consist of four pairs of flagella, the adhesive disc, the median body and the funis [4,5].The adhesive disc and flagella are essential for trophozoite mobility, cell division and proliferation, as well as attachment to epithelial cells in the small intestinal mucosa [6,7].The parasitic G. lamblia trophozoites in the small intestine can cause diarrhea, which is mainly explained by the parasite relying on its adhesive disc to attach to the surface of small intestinal epithelial cells, assisted by flagella.As a result, the intestinal microvilli are damaged directly, which causes diffuse dysfunction of microvilli and local inflammation.Eventually, diarrhea occurs as a result of nutrient and water absorption disorder [8].Therefore, the cytoskeleton plays a critical role in the pathogenesis of G. lamblia infection [9,10].
It was reported that the cytoskeletal proteins of G. lamblia mainly include giardin, dynein, tubulin, actin and several related proteins [5].Among them, giardin is a unique component of G. lamblia cytoskeleton.Crossley and Holberton first reported that giardin is a unique component of G. lamblia cytoskeleton in 1983.Giardin is divided into four types, including α, β, γ, and δ-giardin [11,12].Alpha-giardin is the largest family, with 21 variants with molecular weights ranging from 29 to 38 kDa.The α-giardin variants are named by Arabic numbers preceded by the Greek letter "α", with a "-" inserted between them.Alpha-giardin include α-1 to α-6, α-7.1, α-7.2, α-7.3, and α-8 to α-19 [13,14].The expression of α-giardin is strictly regulated, and there are significant differences in the levels of expression of its members [15] with distinct subcellular localizations, suggesting that each member may have different significance in the survival of G. lamblia [16].Currently, studies assessing giardin's functions are scarce.
Alpha-4 giardin is a member of the α giardin family.In a previous study, we prepared a specific antibody against α-4 giardin and identified its localization in G. lamblia trophozoites [17].However, the specific function of α-4 giardin remains unclear.
A given protein does not usually function alone, more or less interacting with other proteinaceous components.It is helpful to assess the functions and mechanisms of unknown proteins by recognizing protein components that interact with the latter.In this study, α-4 giardin was downregulated by morpholinos for biological traits evaluation.A yeast two-hybrid cDNA library obtained from G. lamblia strain C2 trophozoites was screened for interaction partners of α-4 giardin.The interaction between the partner protein and α-4 giardin was confirmed by co-immunoprecipitation and fluorescent colocalization assays.The results provide novel insights into the mechanism of α-4 giardin's biological function.

Parasite Strain
The G. lamblia isolate utilized in these studies (C2), which belongs to Genotype A, was derived from a patient in southwest China [18] Trophozoites were cultured and propagated in modified TYI-S-33 medium.Subcultures were performed every 3 days [19].

Effect of α-4 Giardin on Parasite Growth
To evaluate the effect of α-4 giardin on parasite growth, α-4 giardin morpholino transfected trophozoites were cultured with a density of 50,000 parasites/mL in TYI-S-33 medium at 37 ℃ for 24, 48 and 72 h.Mispair morpholino transfected and water transfected G. lamblia trophozoites were used as controls, respectively.The cells were harvested by cooling the culture tubes and the cells were counted using a Neubauer chamber.

Effect of α-4 Giardin on Adherence
To evaluate the effect of α-4 giardin on adherence, an adherence inhibition assay was performed as previously described [21].Briefly, 50,000 parasites/mL were grown at concentrations and time described above.After incubation, medium containing non-adherent cells was removed and kept on ice, tubes were filled with cold phosphate buffered saline (PBS) and placed on ice bath for 30 min to dislodge the adherent cells.The numbers of adherent and non-adherent trophozoites were determined by counting in a Neubauer chamber.The results were expressed as percentage of non-adhered trophozoites in relation to the total number of cells.

Yeast Two-Hybrid Screen
A Matchmaker two-hybrid system (Clontech, Mountain View, USA) was used to screen proteins interacting with α-4 giardin from a yeast two-hybrid cDNA library of G. lamblia strain C2 trophozoites.The bait yeast strain Y187 transformed with pGBKT7-α-4 was cultured in 50 mL SD/-Trp liquid medium at 30 °C until an OD600 of 0.8.The bait yeast strain was collected by centrifugation for 5 min at 1000×g and resuspended in 5 mL SD/-Trp liquid medium, and combined with 1 mL of library strain in a 1-L sterile flask.Culture was performed in 45 mL 2 × YPDA (50 mg/ mL kanamycin) liquid medium at 30 °C with shaking for 22 h.From a drop of the mated culture, fusion was analyzed by microscopy to assess the presence or absence of zygotes.When zygotes were observed, the mated cultures were collected and resuspended in 5 mL 0.5 × YPDA/kanamycin liquid medium, spread on selective media SD/-Leu/-Trp/-His plates, and cultured for 5 days at 30 °C.To reduce false positives, all positive colonies were transferred to new selective media SD/-Leu/-Trp/-His/-Ade and SD/-Leu/-Trp plates for further screening.Clones growing on both plates were inoculated on another SD/-Leu/-Trp/-His/-Ade plate for a second screening.All positive clones were picked and cultured in selective liquid medium (SD/-Leu/-Trp/-His/-Ade/kanamycin) overnight at 30 °C.To estimate the sizes of specific inserts from putative positive clones, PCR was carried out using universal primers for pGADT7.Based on the PCR results, prey plasmids from putative positive clones were extracted using the Easy Yeast Plasmid Isolation kit (Clontech, Mountain View, USA), transformed into E. coli DH5a competent cells, and cultured on LB/Amp plates for sequencing.

Confirmation of Positive Clones of Interest
To eliminate false positives, the library plasmids were cotransferred into yeast cells with the pGBKT7/α-4 bait vector, and spread on a SD/-Leu/-Trp plate.The cultured clones were inoculated on SD/-Leu/-Trp and SD/-Leu/-Trp/-His/-Ade plates, respectively, to assess the interaction between the plasmid encoded protein and the bait protein.In addition, positive (pGBKT7-p53 and pGADT7-T) and negative (pGBKT7 and pGADT7) controls were assessed simultaneously.Clones were selected from each set of plates and inoculated into SD/-Leu/-Trp and SD/-Leu/-Trp/-His/-Ade plates, respectively, and observed for growth.Sequences of putative positive clones were analyzed using BLAST programs at NCBI (http:// www.ncbi.nlm.nih.gov/ BLAST/) and the G. lamblia genome sequence (http:// giard iadb.org/ giard iadb/).

Production of Anti-gEB1 and Anti-α-4 Giardin Antibodies
To produce antibodies specifically against the gEB1 protein, a synthesized antigenic peptide with the sequence AVTKT-SKPGNRSGST which corresponds to residues 135-149 of gEB1 was conjugated with Keyhole Limpet Hemocyanin (KLH) and injected intraperitoneally into rabbits after mixed with Freund's complete adjuvant, followed once weekly by 4 injections of incomplete Freund's adjuvant.Seven days after the last injection, blood was extracted, and the serum was collected and purified by protein A sefinose column (Sangon, Shanghai, China).Anti-α-4 giardin monoclonal antibody was generated by immunizing mice with a synthesized antigenic peptide with the sequence VKHDRKYRK-SIKSDAEAFR corresponding to residues 145-163 of α-4 giardin.The specificity of the antibodies were confirmed by Western blot using the lysate of trophozoites and stored in aliquots at -20℃ until use.

Co-immunoprecipitation
Co-immunoprecipitation analysis was employed to verify the interaction between α-4 giardin and G. lamblia endbinding 1 protein (gEB1).Plasmids pcDNA3.1-FLAG-α-4 and pCMV-Myc-gEB1 were cotransfected into 293 T cells using Lipofectamine 2000 (Invitrogen, Carlsbad, USA).Plasmid pcDNA3.1-FLAG-α-4giardin was cotransfected with pCMV-N-Myc into HEK293T cells and served as a negative control.At 48 h after transfection, the cells were resuspended in lysis buffer, and the lysate was used for coimmunoprecipitation assays employing the anti-FLAG mouse monoclonal antibody (CWBIO, Beijing, China) and Protein A/G Plus Agarose Immunoprecipitation Kit according to the manufacturer's protocol (Sangon, Shanghai, China).The eluted immunoprecipitates and total cell lysates were boiled in SDS loading buffer for 10 min and then subjected to immunoblot analysis using anti-FLAG antibody and anti-Myc antibody (CWBIO, Beijing, China).
For endogenous co-immunoprecipitations, lysates from G. lamblia trophozoites were immunoprecipitated with prepared anti-α-4 giardin antibody as described above, and analyzed by Western blotting with anti-gEB1 antibody.

Immunofluorescence Assays
Trophozoites grown on coverslips were fixed with 4% paraformaldehyde (PFA) at room temperature for 30 min, permeabilized with 0.5% Triton X-100 in PBS (PBS-Triton) for 30 min and incubated with 5% goat serum for 1 h at room temperature.Trophozoites were incubated with mouse monoclonal antibodies against α-4 giardin (1:100) and rabbit polyclonal anti-gEB1 antibodies (1:100), overnight at 4 °C, followed by incubation with Alexa Fluor 488-conjugated goat anti-mouse and RBITC-conjugated goat anti-rabbit secondary antibodies (1:200) (Sangon, Shanghai, China), respectively, for 1 h at room temperature.DAPI was used to stain the cell nuclei at a concentration of 5 ug/mL for 20 min at room temperature.All preparations were preserved using the anti-fade mounting media (Sangon, Shanghai, China) and examined using Laser Scanning Confocal Microscopy Leica SP8 STED 3X system.

Statistical Analysis
All quantified results were presented as mean ± SD.The data analysis was evaluated using GraphPad Prism 8.01 statistical analysis software (GraphPad Software).Statistical comparisons among groups were performed by one-way ANOVA.P < 0.05 was regarded as significant.

Down-Regulation α-4 Giardin for Inhibiting Proliferation and Decreasing Adherence
Morpholinos were introduced into G. lamblia trophozoites by electroporation and then differences were observed between the three types of cells, namely, α-4 morpholino (α-4 MO) introduced, mispair control morpholino (C-MO) introduced and sterile water treated (mock).The ability of morpholino to knock down α-4 giardin was demonstrated by western blot at 24 h after electroporation.The presence of α-4 MO had no observable effect on β-actin expression compared to control.α-4 Giardin in the mock group and C-MO group were expressed at high levels; however, it had decreased by ~ 63% in the cultures treated with 100 μM α-4 morpholino (Fig. 1).
Cell counting were performed using a Neubauer counting chamber to investigate the effects of α-4 giardin knockdown on cellular proliferation and adhesion in G. lamblia trophozoites.The results indicated that downregulation of α-4 giardin can significantly inhibit the proliferation and adhesion of G. lamblia trophozoites at each timepoint (Fig. 1B).The non-adherence of α-4 MO group was increased to ~ 15% after 24 h of electroporation (Fig. 1C), but the maximal adherence inhibition for α-4 MO group was observed at 72 h (~ 16% inhibition), which was significantly higher than mock and C-MO groups (~ 8% and ~ 8.6% inhibition, respectively).

Yeast Two-Hybrid Screen
A yeast two-hybrid cDNA library from G. lamblia strain C2 trophozoites was previously constructed by our laboratory and screened for interaction partners of α-4 giardin by a yeast two-hybrid system.A bait plasmid containing coding region of α-4 giardin was constructed, and indicated that the bait protein had no toxicity in the yeast strain Y187 (Fig. 2A).
To screen for proteins interacting with α-4 giardin, Y187 cells harboring the pGBKT7-α-4 plasmid were used to mate with the constructed yeast two-hybrid cDNA library from G. lamblia strain C2 trophozoites according to the manufacturer's instructions.A highly selective medium was used to screen for interacting proteins.After mating and growth on selection SD/-Trp, SD/-Leu, and SD/-Trp/-Leu media, 4 colonies were cultured on SD/-Leu/-Trp and SD/-Leu/-Trp/-His/-Ade plates, with positive ones selected on SD/-Leu/-Trp/-His/-Ade plates three times.Finally, the selected colonies were cultured in selective liquid medium (SD/-Trp/-Leu/-His/-Ade).Specific inserts for various putative positive clones were amplified by PCR and analyzed by gel electrophoresis.All 4 positive colonies were selected for culture in selective liquid medium (SD/-Leu/-Trp/-His/-Ade/kanamycin) (Fig. 2B).Specific inserts for various putative positive clones were extracted and transformed into E. coli.To eliminate false positives and retest interaction specificity, each of the 4 prey plasmids (pGADT7-X) was cotransformed with pGBKT7-α-4 into the yeast strain Y187, and co-transformants were assessed on SD/-Leu/-Trp/-His/-Ade plates.Of 4 prey putative positive plasmids, clones 1, 3, and 4 could grow on both SD/-Leu/-Trp and SD/-Leu/-Trp/-His/-Ade defective plates, suggesting that there may be interactions between these three clones and α-4 giardin (Fig. 2C).
Sequences of the 3 putative positive genes were analyzed for similarity using the BLAST program at NCBI (http:// www.ncbi.nlm.nih.gov/ BLAST/) against the G. lamblia genome sequence.One of the sequences had no meaningful results.The other two putative interacting proteins were G. lamblia end binding protein 1 (gEB1) and ribosomal protein L21.

Identification and Immunolocalization of α-4 Giardin and gEB1
Althoughα-4 giardin and gEB1 physically interact, it was important to verify that these two proteins are normally expressed in a manner that provides the opportunity to interact in trophozoites.In situ localizations of α-4 giardin and gEB1 were identified by immunofluorescence analysis using anti-α-4 giardin monoclonal antibody and anti-gEB1 polyclonal antibody.In trophozoites, α-4 giardin showed a scattered distribution in the in the cytoplasm.In addition, gEB1 was predominantly expressed in the nuclear membrane and nearby cytoplasm, as well as median body.A similar location was determined (Fig. 4).A Western blot analysis of α-4 giardin knockdown efficiency.inG. lamblia trophozoites.Alpha 4-giardin protein levels were measured using immunoblot assay with antibody anti-α-4 giardin.Beta-actin expression was determined as a loading control for each sample.The bands were quantified and presented as the mean ± SD of three independent experiments (right).Subsequent quantitative analysis revealed that the protein expression level of the α-4 giardin was significantly reduced following morpholino knockdown (**P < 0.01).B Growth rate of G. lamblia trophozoites transfected with α-4 MO is slower than that of C-MO and mock groups at 24 h, 48 h and 72 h.The results represent the mean of triplicate determinations ± SD of a representative experiment (P < 0.01).C Adhension inhibition rate of G. lamblia trophozoites transfected with α-4 MO is significant higher than that of C-MO and mock groups at 24 h, 48 h and 72 h.The results represent the mean of triplicate determinations ± SD of a representative experiment (**P < 0.01)

Discussion
Alpha giardin is the most studied type of giardin by far.Phylogenetic analyses showed that it belongs to homologous analogues of annexin [4], which are Ca 2+ -dependent phospholipid-binding proteins.Annexin is an intracellular protein, and accounts for about 2% of the total protein in the cell.It exists in the cell or binds to the cell membrane or cytoskeleton.Annexin is widely found in various eukaryotic cells.To date, thousands of members of the annexin family have been reported in a variety of biological species.Phylogenetic analyses showed that the annexin family is highly conserved in eukaryotes, with all having a highly conserved central domain, which can reversibly bind to phospholipids in a calcium dependent manner.According to their structures, evolutionary relationships, and locations on the chromosome, annexins can be classified into five families, including A (vertebrates), B (invertebrates), C (fungi and some groups of unicellular eukaryotes), D (plants), and E (protists).Annexins interact with various cell-membrane components involved in the structural organization of the cell, intracellular signaling by enzyme modulation and ion flux, and growth control; they also act as atypical calcium channels and exert many other important cellular physiological effects.However, functional differences among the various members of the annexin family remain puzzling.
Most eukaryotic species have 1-20 annexin genes.For example, humans have 12 annexins; Arabidopsis thaliana has 8, and only 2 ~ 4 are found in Saccharomyces cerevisiae and Caenorhabditis elegans [6].Trichomonas vaginalis, another protozoa, has only one annexin analogue.No annexin analogues have been found in Plasmodium spp.and Trypanosoma spp.However, it is interesting that G. lamblia, a representative of lower eukaryotes, has up to 21 annexin tive plasmids (1-4) grew on SD/-Leu/-Trp/-His/-Ade plates; 5: positive control (pGBKT7/p53 + pGADT7/T transformant); 6: negative control (pGBKT7 + pGADT7 transformant).II, Y187 cotransformed with pGBKT7 and each of the 4 putatively positive plasmids grew on SD/-Leu/-Trp/-His/-Ade plates.III, Y187 cotransformed with pGBKT7-α-4 and each of the 4 putatively positive plasmids (1-4) grew on SD/-Leu/-Trp plates; 5: positive control; 6: negative control.IV, Y187 cotransformed with pGBKT7 and each of the 4 putatively positive plasmids grew on SD/-Leu/-Trp plates analogues, including α giardin.Giardin belongs to category E annexins, with less functional studies.The α giardin family members have some sequence similarities, but are not identical.Previous studies have shown that 21 giardin variants are located in different parts of G. lamblia trophozoites.For example, α-3, α-5 and α-17 giardin proteins are mainly distributed in the ventral adhesive disc, while α-18 and α-20 giardin are mainly located in flagella and the cytoplasm [22]; α-8 giardin is mainly located in the cytoplasmic membrane and flagella [23].α-4 Giardin was mainly found in the cytoplasm and the flagellar root in a previous study by our team.Different subcellular localizations suggest that there may be functional differences for α giardin family members.Assessing why G. lamblia, a primitive eukaryote, has so many annexins, and the functional differences among them is very important in understanding the mechanisms of action of annexins as well as the survival mechanism of G. lamblia.Currently, the specific functions of various α giardin proteins are mostly unknown.In this study, a vivo morpholino was employed to block the expression of α-4 giardin in trophozoites.Morpholino antisense oligonucleotides are common used to transient knockdown of gene expression by blocking translation of a targeted protein, which have been proved to be a simple and effective gene knockdown technique in G. lamblia research.The results showed that downregulation of α-4 giardin could impair the proliferation and adhesion of G. lamblia trophozoites.However, in previous study, downregulation of α-8 giardin also inhibited the proliferation of G. lamblia trophozoites.These results implied that knockdown experiments cannot reflect subtle functional differences among α giardin family members.
Identification of interacting proteins may be an effective approach to detect differences in the mechanisms of action among α giardin family members.Therefore, a yeast twohybrid library containing all cDNAs of G. lamblia strain C2, with a capacity reaching 2.715 × 10 7 CFU, was previously constructed by our laboratory and screened by α-4 giardin bait plasmid in this study.After screening, only two α-4 giardin interacting proteins, EB1 and ribosomal protein L21, were obtained.EB1 is a highly conserved protein in eukaryotes; its N-terminal region has a typical actin binding domain referred to as the CH domain, whereas the EB1 domain at the C-terminal end plays a role in dimerization and binding to EB1-interacting proteins.Under normal conditions, EB1 preferentially binds to fast growing microtubule ends to participate in cell cycle control.It mainly controls the dynamics of the microtubule system and promotes the proper positioning of spindles, which play a very important role in the process of mitosis [24,25].Knockout of the EB1 protein may result in significantly reduced mitosis in G. lamblia trophozoites [26,27].It was previously shown that actin, β-giardin and γ-giardin are also interacting proteins of EB1 [28].
To determine the interaction between α-4 giardin and gEB1 protein, co-immunoprecipitation assay was performed.First, the assay was performed by transfection of exogenous alpha-4 giardin and gEB1.However, common eukaryotic expression vectors are not suitable for gene expression in G. lamblia trophozoites because of the distinctive promoter structure of G. lamblia genes.There was no appropriate expression vector for G. lamblia trophozoites in our laboratory.Considering that eukaryotes have similar protein processing and transport modes, alpha-4 giardin and gEB1 genes were transfected into HEK293T cells through common eukaryotic expression vectors.Furthermore, an endogenous co-immunoprecipitation assay was also performed in G. lamblia trophozoites, which showed the endogenous interaction between α-4 giardin and gEB1.As a result, the interaction between the two proteins was confirmed.
Although α-4 giardin and gEB1 physically interact, it was important to verify that these two proteins are normally expressed in a manner that provides the opportunity to interact in trophozoites.For this aim, specific antibodies against the two proteins were prepared separately and the interaction of α-4 giardin and gEB1 in vivo was further confirmed by the immunofluorescence assay in G. lamblia trophozoites.As shown in the results, there is a partial overlap in the localisation of the two proteins, but not a complete overlap.It is speculated that the interaction between the two proteins may be temporary.Another possibility is that α-4 giardin is only one of many interacting proteins in gEB1, so the localization of α-4 giardin and gEB1 is, therefore, not completely overlapping.Anyway, the immunofluorescence assay has shown the existence of co-localization sites between α-4 giardin and gEB1, which is sufficient to demonstrate the possibility of interaction between the two proteins in vivo.
Ribosomal protein L21 is a constitutive protein of the large ribosomal subunit, and found in the cytoplasm of human cells, participating in embryogenesis [29,30], odontogenesis [31], and the formation of age-related cataracts [32] in humans.However, no studies have confirmed direct interactions between this protein and cytoskeletal proteins.Whether an actual interaction exists between ribosomal protein L21 and α-4 giardin needs further investigation.

Conclusion
Our results indicated that α-4 giardin was involved in proliferation and adhesion in G. lamblia trophozoites, and EB1, a crucial roles in mitosis, was an interacting partner of α-4 giardin.Our work lays the foundation for further investigation of functional mechanism of α-4 giardin.
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Fig. 1
Fig. 1 Effect of α-4 giardin knockdown on G. lamblia trophozoites.A Western blot analysis of α-4 giardin knockdown efficiency.inG. lamblia trophozoites.Alpha 4-giardin protein levels were measured using immunoblot assay with antibody anti-α-4 giardin.Beta-actin expression was determined as a loading control for each sample.The bands were quantified and presented as the mean ± SD of three independent experiments (right).Subsequent quantitative analysis revealed that the protein expression level of the α-4 giardin was significantly reduced following morpholino knockdown (**P < 0.01).B

Fig. 3 Fig. 4
Fig.3Interaction between α-4 giardin with gEB1.A Immunoprecipitation using HEK293T cells transfected with the indicated combination of pcDNA3.1-FLAG-α-4giardin and pCMV-Myc-gEB1.Cell extracts were immunoprecipitated from the transfected HEK293 cells using anti-FLAG antibody and the immunoprecipitated materials were analyzed by anti-Myc antibody.Rabbit and mouse IgG antibodies were used as negative controls in the immunoprecipitation reaction.B Identification of antibodies specificity by Western Blot analysis.M: protein molecular marker; Lane 1: lysate of E. coli Rosetta (DE3) harboring the plasmid pET-28a-gEB1 without addition of IPTG was immunodetected using the anti-gEB1 (1:1000) polyclonal antibody; 2: lysate of E. coli Rosetta (DE3) harboring the plasmid pET-28a-gEB1 after induction by 1 mM IPTG was immunodetected using the anti-gEB1 (1:1000) polyclonal antibody; Lane 3: lysate of G. lamblia trophozoites was immunodetected using the