Study site

The study site is located in the middle-west of the Vakinankaratra region near Ivory (19°33’03’’S; 46°24’37’’E; 908 m asl) on mesozoic sedimentary rocks. Mean annual precipitation and temperature recorded from 2005 to 2020, with an automatic weather station (CIMEL, Electronique, Paris, France) located near the experimental field, were, respectively, 1,291 mm and 23.1 °C. Total annual precipitation from September 2019 to August 2020, corresponding to the cropping season in the present study, was 1,350 mm, showing a normal rainfall pattern. The soil is a sandy loam ferralsol (FAO) comprising 4% clay, 38% silt, and 58% sand. The soil contained 27.2 g kg⁻¹ of C, 2.09 g kg⁻¹ of total N, 540 mg kg⁻¹ of total P and 11 mg kg⁻¹ of available Olsen P. The cation exchange capacity (cobaltihexamine) was 136 cmolc kg^−1, and pH of water was 4.7.

Experimental design

In the previous cropping season, the field was cultivated with homogenous cowpea crops with no fertilization. The legume residues after grain harvesting were left on the soil. Our field experiment was conducted in the 2019–2020 cropping season with a complete split-plot design with four blocks and three factors, rice variety (V), phosphorus fertilization (P), and AMF inoculation (I). To make field operations easier, PI treatments combining P supply and AMF inoculation were applied in the main plots using four randomly allocated treatments: control (00), inoculation alone (0I), P alone (P0), and inoculation and P (PI). The V factor was applied in subplots with four randomly allocated varieties. The experiment totaled 64 plots. The plot size was 10.8 m² (width 3.6 m and length 3 m).

Plant and AMF materials

Four rice varieties promoted by national research (Rakotoson et al., Reference Rakotoson, Dusserre, Letourmy, Ramonta, Cao, Ramanantsoanirina, Roumet, Ahmadi and Raboin2017) were used with the following main characteristics (Table 1): The Nerica 4 variety (N4), an interspecific crossbreeding of Oryza sativa group japonica × O. glaberrima parents. This variety is popular and used in different African countries (Diedhiou et al., Reference Diedhiou, Mbaye, Mbodj, Faye, PIgnoly, Ndoye, Djaman, Gaye, Kane, Laplaze, Manneh and Champion2016; Wissuwa et al., Reference Wissuwa, Gonzalez and Watts-Williams2020). FOFIFA 182 (F182) and WAB 880-1-32-1-1-P2-HB-1 (WAB) were new varieties, both improved from Nerica 4. FOFIFA 185 is an intraspecific variety with Oryza sativa group japonica parents.

Table 1 Main characteristics of the four rice varieties tested in the experiment

The commercial inoculant AGTIV PTB297 © was provided by Premier Tech company. This inoculant contained a Rhizophagus irregularis strain with an expected colony formation of 6,400 g⁻¹ units in an inert kaolinite matrix.

Soil and crop management

No pesticide was applied so as not to interfere with either native or inoculated AMF. The plots were plowed by hand to a depth of 15 cm, from November 4–9, 2019. The rice was sowed on November 19 after a cumulated rainfall of 36.5 mm measured starting on November 10. Rice holes were dug by hand with an angady (local spade) at 20 cm intervals using a string to be sure that both the holes and the rows were evenly spaced.

In the P0 and PI treatments, 20 kg ha⁻¹ of P₂O₅ was applied in the form of a triple superphosphate fertilizer (46% P₂O_5, 14% Ca). Six granules of triple superphosphate fertilizer were carefully placed in each hole, corresponding to around 0.18 g per hole and 47 g per plot. Seven seeds were then placed in each hole. In the 0I and PI treatments, the inoculant was adjusted with weight grain by seed coating to obtain 16 spores per grain. For each variety, 70 g of seeds per plot were mixed with 5 ml of tap water.

A farmyard cattle manure previously homogenized by thorough mixing was applied in all the treatments using a standard quantity per hole to reach a quantity of 5 tons per ha based on dry matter (DM) weight (75% DM at application time, 7 kg per plot). The nutrient contents of the cattle manure were 0.83% N, 9.88% C, 0.22% P, 1.47% K, 0.70% Ca, and 0.38% Mg.

In order to characterize the environment of the bioinoculant, in situ soil pH was recorded 7 days after sowing (DAS) using a Hanna Instruments 99121 portable meter and an electrode inserted to a depth of 5 cm after saturating the soil with deionized water. In rice holes, an increase of around 0.6 pH unit was observed, i.e. 5.3 in rice holes thanks to localized manure application compared to rice inter-rows in inter-rows without manure (pH of 4.7).

Three applications of urea (46% N) were manually and gently made in all the treatments 40, 65, and 88 DAS each at a rate of 30 N units (total of 90 kg ha⁻¹). Hand weeding was performed 35 and 58 DAS. Rice was harvested at maturity on March 20 (F185), March 28 (N4 and F182), and April 1 (WAB).

Plant analysis

At 60 DAS corresponding to tillering, plants (shoot and roots) were sampled from two rice holes chosen at random in rows bordering the central plot to measure the number of tillers, shoot DM, and shoot nitrogen (N) and P content on representative samples. At maturity, i.e., from 110 to 125 DAS, we recorded the total number of tillers, the DM in the straw and grain on a 4.84 m² area in the central part of the plot. Subsamples of straw and grain were kept for N and P analysis. Total N content was measured with a CHNS microanalyzer (Flash 2000 Series, CHNS/O 122 Analyzers Thermo Scientific, IRCOF, France). Total P content was also measured following mineralization in a microwave oven using 65% nitric acid. Colorimetric dosage was then performed using the malachite green method (Ohno and Zibilske, Reference Ohno and Zibilske1991).

AMF root colonization

Root systems of rice plants harvested in the field at 60 DAS were washed with tap water. All coronal roots were cut and 30 fragments of lateral roots were randomly selected, carefully washed and fixed in 20 ml of 70% ethanol before transport to the laboratory. The fragments were then incubated for 12 hours in a 10% KOH solution, rinsed twice with tap water and immediately stained with 8% of blue Shaefer ink diluted in vinegar (5% acetic acid) (Wilkes et al., Reference Wilkes, Warner, Edmonds-Brown, Davies and Denholm2020). Endomycorrhizal structures were stained by immersion in a water bath for 30 minutes at 70°C. Roots were de-stained with acetic-glycerol for 30 minutes. Five mycorrhizal parameters of 1-cm long root segment were assessed under the microscope (Olympus BX 41), using a semi-subjective scoring method at a magnification ranging from ×40 to ×200. Each root segment required 10 observations. The structures of AMF infection (intracellular hyphae, vesicles, arbuscules) were assessed using six scores with their percentages in parentheses, 0 (0%), 1 (0–1%), 2 (1–10%), 3 (10–50%), 4 (50–90%), 5 (90–100%), with n1 = number of fragments rated 1, n2 = 2, n3 = 3, n4 = 4, n5 = 5. Arbuscular abundance was assessed using four scores, 0 (no arbuscular colonization), 1 (low abundance), 2 (medium abundance), 3 (high abundance), with A1 = number of fragments scored 1, A2 = 2, A3 = 3. The five mycorrhizal parameters were computed as % according to the methodology used by Vallino et al., Reference Vallino, Fiorilli and Bonfante2014 and Campo et al., Reference Campo, Martín-Cardoso, Olivé, Pla, Catala-Forner, Martínez-Eixarch and San Segundo2020:

• The AMF frequency of the root system,

(1) $$F\;\left( \% \right) = \left( {MF/30} \right)100$$

• The AMF Intensity of the root system,

(2) $$M\;\left( \% \right) = \left( {95n5 + 70n4 + 30n3 + 5n2 + n1} \right)/30{\rm{\;}}$$

• m, as the AMF Intensity of the mycorrhized fragments,

(3) $$m\;\left( \% \right) = \;M\;\left( \% \right)\left( {30/MF} \right)$$

• The arbuscular abundance of the mycorrhized fragments,

(4) $$a\;\left( \% \right) = \left( {100mA3 + 50mA2 + 10mA1} \right)/100$$

• A, as the arbuscular abundance in the root system,

(5) $$A\;\left( \% \right) = a\left( {M/100} \right)$$

where:

MF: number of mycorrhized fragments

(6) $$mA3 = \left( {95n53 + 70n4A3 + 30n3A3 + 5n2A3 + n1A3} \right)/MF100/m$$

(7) $$mA2 = \left( {95n5A2 + 70n4A2 + 30n3A2 + 5n2A2 + n1A2} \right)/MF100/m$$

(8) $$mA1 = \left( {95n5A1 + 70n4A1 + 30n3A1 + 5n2A1 + n1A1} \right)/MF100/m$$

Data analysis

All statistical analyses were performed in R (R-4.1.1). The packages lme4 and lmerTest were used with a p-value threshold set at 5% for tests of linear mixed effects model fit. Means were compared according to the least significant difference (LSD) with Fisher’s LSD test with a probability level of 5% with the stats package. Normality and variance assumptions were tested with the Shapiro test (stats package) and the Levene test (car package). ANOVAs were used with the V, P, and I factors as fixed effects, and the Block and PI × block (constraint of the split-plot design) as random effects. For the mycorrhizal parameters expressed in percentages, data were transformed using arcsin square root function. The packages FactoMineR and factoextra were used to perform a principal component analysis (PCA) with rice growth variables as active (n = 11), and mycorrhizal parameters (n = 5), as additional variables.