Bird management, experimental design and diets

In the present study, 38-week-old Hyline Grey laying hens (n 384) with similar performance (laying rate: 88·65 (SEM 1·79) %; body weight: 1·42 (SEM 0·07) kg) were randomly allocated to four treatments: a control group fed without additional Zn supplementation in premix, the first experimental group fed lowered level of organic Zn as Zn-Met (40 mg Zn per kg of diet) (rate of chelation: 99·0 %, purity: 96·00 %, 16·00 % of Zn content, 80·00 % of Met; Novo International Trading Co., Ltd), the second experimental group fed recommended levels of organic Zn as Zn-Met (80 mg Zn per kg of diet) and the group receiving Zn in 100 % of daily recommended dose from ZnSO₄ monohydrate (80 mg Zn per kg of diet) (≧99·00 % in purity; Sinopharm Chemical Reagent Co. Ltd). Each of the groups consisted of six replications in four different cages (four birds per cage). The size of each cage (equipped with two nipple drinkers and one feeder) was 50 × 60 × 60 cm³. An enclosed, ventilated and conventional house with 16 h lighting was provided for all laying hens to keep them in the same environmental conditions. Feed and water were offered ad libitum. The experiment lasted 12 weeks, consisting of a 2-week adaption period and a 10-week experimental period. During the adaption period from 38 to 40 weeks of age, all laying hens were fed the normal diet with 80 mg/kg Zn (China feed standard) to make them similar with regard to healthy laying performance.

The basal maize–soyabean meal diet (Table 1) was formulated to meet or exceed the requirements for laying hens (National Research Council, 1994)⁽²¹⁾. Different Zn sources were supplemented in the premixes. Differential contents of Met in these groups were caused by addition of Zn-Met in premix, which was corrected by the addition of extra Met (dl-methionine) in the premix. Hence, all nutrients were kept at the same levels except for Zn content that met the nutritional requirements in the basal diet, which was in accordance with NY/T 33-2004 (Chicken Feeding Standard, Agricultural Industry Standard of the People’s Republic of China). Approximately 200 g of each diet was collected and stored at −20°C for analysis of the Zn content according to the method of atomic absorption spectrometry using an atom absorption spectrophotometer. The analysed Zn contents in the four experimental diets were 24·99, 65·35, 105·33 and 105·22 mg/kg for control, Zn-Met (40 and 80 mg/kg), and ZnSO₄, respectively.

Table 1. Composition of the experimental basal diet

* The premixes provided the following per kg of diet: vitamin A 7500 IU, vitamin D₃ 2500 IU, vitamin E 25 mg, vitamin K₃ 2·5 mg, vitamin B₁ 1·5 mg, vitamin B₂ 4·5 mg, vitamin B₆ 3 mg, vitamin B₁₂ 0·02 mg, niacin 25 mg, folic acid 1·1 mg, calcium pantothenate 8 mg, biotin 0·12 mg, choline chloride 400 mg, Cu 20 mg, Mn 60 mg, Fe 90 mg, iodine 0·8 mg, Se 0·3 mg.

† The premix in the control diet provided per kg of diet: 0 mg of Zn/kg; the premixes in another two groups provided per kg of diet: 40, 80 mg Zn/kg as Zn-methionine (Zn-Met), respectively; the premix in the last group provided per kg of diet: 80 mg Zn/kg as zinc sulphate monohydrate. Different Zn sources were supplemented in the premixes. Differential contents of methionine in these groups were caused by the addition of Zn-Met in the premix, which was corrected by the addition of extra methionine (dl-methionine) in the premix. Hence all nutrients were kept at the same levels except for Zn content which met the nutritional requirements in the basal diet, which was in accordance with NY/T 33-2004 (Chicken Feeding Standard, Agricultural Industry Standard of the People’s Republic of China).

‡ Metabolisable energy based on calculated values; others were analysed values.

Sample collection

At the end of the experiment, thirty-six eggs from each treatment group (six eggs per replication and six replications per treatment) were randomly collected at 5-week and 10-week experimental periods for egg quality determination as reported previously^{(Reference Zhang, Wang and Zhang8)}. Twelve hens from each treatment group (two hens per replication) were randomly selected and marked. After 12-h feed withdrawal (water was offered ad libitum), hens were killed humanely by carbon dioxide asphyxiation. The ovary, magnum, and ESG samples were collected immediately. A set of tissue sub-samples was snap-frozen in liquid N₂ and then stored in −80°C for the mRNA level analysis. Another set of sub-samples was kept on ice and stored at −20°C for subsequent measurements of Zn content, Ca, P, total protein (TP) and albumin (Alb) levels as well as the activities of alkaline phosphatase (ALP) and CA. Blood samples collected from the wing vein were centrifuged for 10 min (3000 g ) to separate out serum. Pure serum samples were aspirated by pipette, stored in 1·5-ml tubes at −80°C until analyses and thawed at 4°C before analysis. All serum samples from two birds in each replicate were pooled into one sample in equal ratios before analysis as previously reported by Liao et al. ^{(Reference Liao, Li and Zhu22)}.

Egg quality determination

Eggshell thickness was measured without membrane using a digital micrometre at three different points (air cell, sharp end and any side of the equator) and estimated by the average of three different thickness measurements from each egg^{(Reference Xiao, Zhang and Wu23,Reference Yilmaz Dikmen, Sözcü and İpek24)} . Egg weight, eggshell strength, albumen height, yolk colour and Haugh unit were measured using an Egg Quality Analyzer (DET-6000; Nabel Co., Ltd)^{(Reference Li, Zhang and Gong25)}. After egg quality determination, yolk and egg white were separated and placed in 50 ml tubes. The eggshell, egg white and egg yolk were collected and frozen (at −20°C) for further analysis.

Eggshell ultrastructure and energy-dispersive X-ray spectroscopy determination

The eggshell collected was washed with distilled water to remove the dirt and the inner shell membrane and then dried at room temperature (25 ± 2°C) for at least 48 h^{(Reference Dunn, Rodriguez-Navarro and Mcdade26)}. Three parts of sample peels from the equator were separated and prepared for field emission scanning electron microscope (SU8010) analysis. Two parts of samples (0·5–1 cm²) were used for the analysis of the external and internal surface of the shell, the third part was used for the assessment of the transversal surface. The samples were glued on an aluminium support (stub), metalized with gold and analysed in the electron microscope^{(Reference Stefanello, Santos and Murakami20)}. For the internal surface analysis, the fibre diameter and fibre gap area were measured using the field emission scanning electron microscope ruler. For the transversal surface analysis, the effective total thickness (combined mammillary layer, palisade, vertical crystal and cuticle sections, μm), the mammillary thickness (μm), the palisade layer thickness (μm) and width of the mammillary knobs (μm) were measured using the field emission scanning electron microscope ruler^{(Reference Dunn, Rodriguez-Navarro and Mcdade26)}. The percentage of the palisade layer thickness and the mammillary thickness were obtained by calculating the percentage of the thickness of each layer to the effective total thickness. Five scanned images were obtained from each sample (six samples per group) using 200× magnification (200 μm, external and internal surface) and 100× magnification (500 μm, transversal surface). Furthermore, the eggshell peels (six samples per treatment) without metallisation by gold were analysed for elemental composition and distribution with an Oxford energy-dispersive X-ray spectroscopy operated at 20 kV and at a working distance (WD) of 20 mm. The energy-dispersive X-ray spectroscopy was calibrated using a pure Co sample operated at 20 kV and at WD 20 mm. The spectrum of elemental peaks was cross examined and data values (relative atomic weight percentages) were normalised. The determination of energy-dispersive X-ray spectroscopy contained line scan and mapping scan of transversal surface of eggshell at a magnification of 200× (200 μm). The same area was determined in transversal surfaces of all groups and contained all kinds of layers in eggshell (average the testing values of repeated measurements).

Zinc contents in eggshell, egg white, egg yolk, serum and eggshell gland

Eggshells were ground to a fine powder, then ashed (550°C, for 14 h) and solubilised in 10 ml hydrochloric acid (6 M) and 30 ml of demineralised water at a high temperature using a sand heater (300°C for 15 min). After filtration (Whatman filter), the volume was increased to 50 ml with demineralised water prior to analysis, according to the method of Gheisari et al. ^{(Reference Gheisari, Sanei and Samie27)}; egg white or yolk was defrosted, mixed and 0·5 g was placed in a plastic high-pressure tube for digestion (7 ml of nitric acid and 2 ml of hydrochloric acid) using an organic program. After cooling, the samples were transferred to 100 ml flasks and brought to 100 ml volume with deionised water for the homogenisation^{(Reference Rubio Zapata28)}; Zn contents in serum, ovary, magnum and ESG were measured according to the method of Chen et al. ^{(Reference Chen, Hogstrand and Luo29)}. Flame atomic absorption spectrophotometry was used in the determination.

Activities of carbonic anhydrase and alkaline phosphatase, the concentrations of calcium, phosphorus, total protein and albumin

The ESG was homogenised in 10 % (w/v) ice-cold physiological saline and then centrifuged for 10 min at 4°C (3000 g ). The supernatant collected and the serum were used to determine the concentrations of Ca, P, TP and Alb and the activities of ALP using analysis kit (Nanjing Jiancheng Bioengineering Institute), and CA activity was measured by ELISA kit (Shanghai mlbio Institute). A microplate reader (Bio-tek ELX800; Biotek Instruments, Inc.) was used in the determination.

RNA extraction, reverse transcription and real-time quantitative PCR

Total RNA was extracted from ESG using Trizol reagent (Invitrogen) according to the manufacturer’s instruction. The concentration of each extracted RNA sample was determined using a Nano Drop Spectrophotometer (ND-2000; Gene Company Ltd), and the integrity of the RNA was checked using denatured RNA electrophoresis. A total of 1 μg RNA was used to obtain complementary DNA by reverse transcription using the HiScript α Q RT SuperMix RT (Vazyme). Real-time quantitative PCR reactions were performed on an ABI 7500 real-time quantitative PCR system with a 10-μl reaction volume containing 5 μl of 2 × ChamQ^TM Universal SYBR-Green qPCR Master Mix (Vazyme), 0·2 μl of 10 µM each of forward and reverse primers, 1 μl diluted complementary DNA template (10-fold) and 3·6 μl double-distilled water. The primer sequences for osteopontin (OPN), ALP, CA, ovocleidin-17, ovocleidin-116, Ca-binding protein-d_28k (CaBP-D_28k) and β-actin are given in Table 2. The protocol of PCR is as follows: denaturation at 95°C for 30 s, followed by 40 cycles of 95°C for 10 s and 60°C for 30 s. All reactions were performed in duplicates and each reaction was verified to contain a single product of the correct size using agarose gel electrophoresis. The 2^−ΔΔCT was used to calculate the mRNA level of each target gene^{(Reference Livak and Schmittgen30)}. The internal reference genes (β-actin) were used to normalise the expression level of the targeted gene.

Table 2. Primers used for real-time quantitative fluorescence PCR analysis

OPN, osteopontin; ALP, alkaline phosphatase; CA, carbonic anhydrase; OC-17, ovocleidin-17; OC-116, ovocleidin-116; CaBP-D_28k , Ca-binding protein-d_28k.

Calculations

Total Met content of premix (2 %) was calculated ((0·34–0·24 %)/5 %) on the basis of removing the Met content (0·24 %) in the maize, soyabean meal and fishmeal from the criteria of Met (0·34 %).

Addition of extra Met in the premix (g/kg) = 2 % × 10³ – Zn addition in premix (g/kg) × quality fraction of Met in Zn sources (80 %).

Statistical analyses

The results were presented as means with standard errors and analysed statistically by one-way ANOVA using SPSS 20.0 except the percentage of relative atomic weight in transversal surface of eggshell (means and standard deviation). Differences among all treatments were separated by the Tukey test for multiple comparisons. The Pearson correlation test (two tails) were used to analyse and examine the relationship between eggshell strength and ultrastructure-related parameters for the 80 mg/kg Zn-Met group. Values of P < 0·05 were considered significant. All the graphs were made using the GraphPad Prism 5.01.