Abstract
Pasteurizing donor human milk inactivates bacteria that may be of concern to the preterm infant. However, current practice for Holder Pasteurization (62.5°C for 30 min) is detrimental to the bioactivity of human milk. An experimental pasteurizer was used to determine the maximum temperature at which 90% of secretory IgA, lysozyme, and lactoferrin were retained and whether this temperature was capable of inactivating five common bacterial contaminants. The retention of these proteins was also compared using a commercially available bottle immersion or holding chamber system. After pasteurization at 62.5°C for 30 min, the retention across all three systems was 72.3 ± 3.6%, 21.8 ± 3.3%, and 39.4 ± 11.5% for sIgA, lactoferrin, and lysozyme, respectively (n = 22). The retention of all three proteins was at least 90% when human milk was pasteurized at 57°C for 30 min, and this temperature was also effective at removing 99.9% of all inoculated bacterial species. In addition, human milk that was pasteurized in the experimental system had a significantly higher proportion of lysozyme compared with samples pasteurized in the bottle immersion system. These findings suggest that optimizing pasteurization temperature and improving pasteurizer design enhances the quality of pasteurized donor human milk.
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Main
Pasteurized donor human milk (PDHM) is considered to be the best alternative to mother's own milk (MOM) for feeding preterm infants, because it contains additional protective and developmental factors not found in infant formula (1). During the expression and collection of human milk, microbial contamination can occur and therefore DHM is pasteurized to prevent transfer of pathogens to the infant.
Current pasteurization methods use simple heating protocols to decrease the level of bacterial contamination to noninfectious levels. Current Australian guidelines (2), as well as the Human Milk Banking Association of North America (HMBANA) and the United Kingdom Association for Milk Banking (UKAMB; 3,4), recommend that human milk should be pasteurized using the Holder Pasteurization method, whereby the monitored temperature of the human milk should not fall below 62.5°C for 30 min. It is also recommended that human milk containing a microbial load greater than 1 × 105 colony-forming units/mL (CFU/mL), bacterial species capable of producing heat-stable enterotoxins, or any pathogens should be rejected (2–4). It is likely that, historically, these recommended pasteurization regimes were adopted from the dairy industry where these conditions were required to inactivate the most heat-resistant, nonspore-forming human pathogens, Mycobacterium tuberculosis and Coxiella burnetti (5). The major purpose of pasteurization in the dairy industry is to prevent the transfer of such pathogens to the consumer and increase shelf life (6), whereas less concern is given to the nutritional changes to the milk that may occur during pasteurization. These pasteurization conditions may not be ideal for human milk, where the retention of bioactivity is highly desirable for sick and preterm babies.
Inevitably, the mechanism of thermal inactivation of bacteria during pasteurization also results in considerable loss of beneficial proteins present in human milk. This can be attributed to the “broad action” of heat that disrupts cell membranes and proteins through thermally induced denaturation (7). Typically, Holder Pasteurization can reduce the function of the immunoprotective proteins, such as secretory immunoglobulin A (sIgA), lactoferrin, and lysozyme, as much as 80% (8–10). Although clinical data suggests that PDHM is as protective in the prevention of necrotizing enterocolitis in the preterm infant as MOM (11), these studies demonstrate the need for a re-evaluation of human milk pasteurization conditions in the context of maximizing the retention of bioactive components.
Human milk pasteurizer design is an additional issue that must be considered. Most human milk pasteurizers submerge bottles of DHM in a heated water bath for the required time, followed by immersion in a chilled water bath until the milk has returned to the desired temperature. Although such systems are able to process a large volume of human milk, the length of time required to heat the milk to the desired temperature (lag time) is often either equivalent to or just short of the holding time. Furthermore, the lack of mixing of the human milk during pasteurization can often result in fat separation and clumping, making it difficult to resuspend in the milk. Both of these issues can be potentially resolved using a semiflow-through system that heats the milk quickly and also mixes it. This study compared the effectiveness of these two different designs in relation to the retention of immunologic proteins (sIgA, lactoferrin, and lysozyme) of human milk. A third experimental pasteurizer was used to determine the optimal pasteurization conditions for protein retention and the effectiveness of these conditions on inactivating common bacterial contaminants found in DHM.
METHODS
Samples.
Samples of human milk used for studying the effects of pasteurization were obtained from the Perron Rotary Expressed Milk Bank (PREM Bank), King Edward Memorial Hospital, Subiaco, Western Australia. All donors gave written consent for their donations to be used in research, and this study was approved by The University of Western Australia ethics review board.
Holder Pasteurization.
Human milk samples were pasteurized using the Holder Method (62.5°C for 30 min) in three different systems. The T30 (Sterifeed, UK) is a bottle immersion-type pasteurizer, wherein 11 bottles containing 250 mL of DHM are submerged in a heated water bath for the required time and then cooled by transferring the bottles to a chilled water bath. The Human Milk Pasteurizer (Saurin Industries, Australia) pumps 750 mL of DHM through a heating coil and into a holding chamber, where it is held for the required time and temperature. The milk is then pumped through a cooling coil and collected for dispensing. Because the temperature resolution of the bottle immersion and holding chamber pasteurizers was ±1.5°C and ±0.5°C, respectively, the actual pasteurizer temperature was adjusted, so that a minimum holding temperature of 62.5°C was maintained.
For the purpose of optimizing pasteurization conditions, an experimental pasteurizer was designed specifically for this study (Carag AG, Switzerland). The experimental pasteurization system was simplistic and used a precision water bath (Huber AG, Germany) capable of maintaining temperatures ±0.1°C of the desired temperatures. Human milk was pasteurized by injecting 50 mL of chilled human milk into a 3-mm diameter stainless steel coil attached to the lid of the water bath. The coil was then submerged into the precisely heated water bath. The temperature of the milk was monitored indirectly using a pair of type K thermocouples (sampling rate of 1 Hz) mounted 1.5 mm apart in a separate 3-mm diameter stainless steel coil filled with water to simulate the thermal characteristics of human milk. Both these coils were attached to the lid of the water bath, so that they could be submerged simultaneously into the water bath for the desired period of time (Fig. 1). The thermocouples were mounted in this way, so that simultaneous measurements of the inside surface of the stainless steel coil and the temperature at the center of the diameter coil could be recorded. After the desired pasteurization time, the coil containing the milk was transferred to insulated container connected to a cooling system. After the temperature of the milk reached 10°C, the milk was decanted from the coil, and samples were taken for further analysis. Temperature data were acquired via a data acquisition system (Delta Ohm, Italy) connected to a personal computer, and subsequent analysis was performed using DeltaLog9 version 2.4 software (Delta Ohm).
Measurement of protein retention.
The sIgA and lactoferrin content of human milk samples were quantified by the sandwich ELISA method as previously described (12). All antibodies and standards were purchased from MP Biomedicals Australasia (New South Wales, Australia). Lysozyme content of human milk samples was quantified using a Human Lysozyme enzyme immunoassay (EIA) kit (Biomedical Technologies, Inc., MA) according to manufacturer's instructions.
Bacteriology.
Five bacterial species were chosen for this study on consultation with the microbiology laboratory that routinely screens samples of human milk donated to the PREM Bank. Lyophilized preparations of Staphylococcus aureus (ATCC 6538), Enterobacter cloacae (ATCC 27508), Bacillus cereus (ATCC 10702), and Staphylococcus epidermidis (ATCC 12228) were obtained from the American Type Culture Collection, VA. An overnight culture of Escherichia coli strain K12 (ATCC 14948) was obtained from Southern Biologic, New South Wales, Australia. E. coli and S. epidermidis were cultured as suspensions in nutrient broth, plated on nutrient agar, and incubated at 37°C. E. cloacae and B. cereus were cultured as suspensions in nutrient broth, plated on nutrient agar (Southern Biological), and incubated at 30°C. S. aureus was cultured as a suspension in Tryptic Soy Broth (BD Biosciences, CA) and plated on Tryptic Soy Agar (BD Biosciences, CA) at 37°C. Bacterium suspension cultures were enumerated using the OD method (13) measured with a spectrophotometer (Biotek Pty Ltd, VT) at 600 nm. For pasteurization, triplicate 50 mL samples of either the human milk or the appropriate nutrient media were inoculated with bacterial suspension to achieve a minimum concentration of 1 × 105 CFU/mL and pasteurized as described above using the experimental pasteurizer. To determine the decimal reduction time (D value) of each bacterial species inoculated into the human milk or nutrient media during pasteurization, samples were taken at 0, 2.5, 5, 7.5, 10, 15, 20, 30, and 40 min, aliquots (5–100 μL) plated on the appropriate nutrient agar, and CFU/mL enumerated 24 h later after incubation under the above conditions.
Statistical analysis.
All averaged data are presented as mean ± SD. ANOVA with Tukey-Kramer post hoc test (GraphPad InStat V3.0; GraphPad Software, Inc.) was used to compare mean values of groups of samples to determine the presence of a significant difference (p < 0.05). Graphical modeling of protein retention levels and rates of bacterial inactivation during pasteurization were performed using SigmaPlot 11.0 (Systat Software, Inc., CA).
RESULTS
Effect of heating time during Holder Pasteurization on the retention of human milk immunologic proteins.
Although there was variation in the concentrations of the individual proteins measured before pasteurization, the proportion of each protein retained after pasteurization was relatively consistent across all three pasteurization systems (Table 1). Secretory IgA had the greatest level of retention ranging between 68.5 and 72.9% (n = 22). Lysozyme was the next greatest retained protein between 32.8 and 52.5% (n = 22), and lactoferrin was the least retained protein in the range of 18.3 to 24.8% (Table 1; n = 22). There was no significant difference between the proportion of sIgA and lactoferrin that was retained as a result of pasteurizing using the different systems. However, significantly greater lysozyme was retained (p < 0.01) in the human milk that was pasteurized using the experimental pasteurizer (n = 6) compared with the bottle immersion pasteurizer (n = 10).
Considerable variation in lag time occurred between the three pasteurization systems, with the bottle immersion system requiring 30 min and the holding chamber system requiring 15 min to heat the milk to the 62.5°C. Comparatively, the experimental pasteurization system allowed for rapid heating of the milk in an average of 45.3 ± 2.6 s (n = 6) with excellent maintenance of holding temperature, producing an ideal heating profile (Fig. 2A). On closer inspection, however, it is apparent that the majority of the lag time was associated with increasing the temperature of the milk from 59.5 to 62.5°C (Fig. 2B). There was also a considerable difference in heating rates at the center and the inside surface of the coil, suggesting that a temperature gradient was generated across the 3-mm diameter of the stainless steel coil in which the human milk was pasteurized (Fig. 2B).
Optimal Holder Pasteurization temperature for maximizing the retention of immunologic proteins.
By using the precision temperature control of the experimental pasteurization system, it was possible to accurately quantify the retention of each protein in relation to time at specific pasteurization temperatures in 1°C increments (Fig. 3). The change in protein retention over time was quantified by calculating the rate of individual protein loss from the mean retention values of each protein (n = 6). Under currently accepted Holder Pasteurization conditions (62.5°C for 30 min), protein loss was 1.6% reduction of protein per min for sIgA, 1.7% per min for lysozyme, and 2.4% per min for lactoferrin. Reducing the temperature to 60°C decreased the rate of protein loss for sIgA and lactoferrin (0.9%/min and 1.9%/min, respectively), but it was less pronounced for lysozyme (1.6%/min). At 59°C, protein loss rates were slightly less for sIgA at 0.6%/min and lactoferrin at 1.7%/min, whereas lysozyme loss fell to 1.4%/min. Further lowering of the pasteurization temperature to 58°C resulted in a protein loss rate for lactoferrin (1.4%/min), with a decrease in protein loss for sIgA (0.5%/min) and lysozyme (1.3%/min). For all three proteins measured, the highest rate of protein retention occurred at 57°C (0.2%/min for sIgA, 0.4%/min for lactoferrin, and 0.2%/min for lysozyme). At this temperature, the rate of protein retention was either similar or identical to what occurred at 40°C (0.2%/min for all three proteins). This decreased rate of protein loss resulted in the retention of all three proteins at levels greater than 90% at all time points measured.
Effect of reducing pasteurization temperature on the inactivation kinetics of common bacterial contaminants found in DHM.
For all bacterial species tested, thermal treatment at 62.5°C resulted in a greater rate of reduction in viable cell number than at 57°C. Pasteurization at 62.5°C for 20 min reduced the numbers of all bacterial species by at least 99.9%, whereas 30 min at 57°C was needed to achieve the same results (Fig. 4). Susceptibility to the pasteurization treatment was found to be dependent on the pasteurization temperature (Table 2). As determined from the decimal reduction values (D), S. aureus exhibited the greatest heat resistance, followed by B. cereus and Enterobacter cloacae, whereas E. coli and S. epidermidis were the least heat resistant at the higher temperature. Reducing the pasteurization temperature appeared to alter the thermal resistance of the bacterial species, with E. coli demonstrating the greatest heat resistance, whereas S. aureus, E. cloacae, S. epidermidis, and B. cereus displayed similar thermal resistance at this temperature.
In all cases, the rate of cell number reduction was less in DHM compared with the nutrient medium. This was more evident at 57°C than at 62.5°C, although there was little difference observed for S. epidermidis, B cereus, and S. aureus at the higher temperature.
DISCUSSION
The three antimicrobial proteins measured in the current study constitute approximately a third of the total protein in human milk and make an important contribution to the antibacterial activity of the milk (14). Despite the large range (e.g. sIgA ranged 0.9–2.3 g/L) in protein content of human milk samples pasteurized in the different systems, protein retention was similar across all three pasteurization systems (Table 1). Furthermore, the proportion of sIgA and lactoferrin retained after pasteurization was similar to previous studies (15,16).
The optimal temperature (of those tested) for the greatest retention of immunologic proteins in human milk was 57°C. This finding was notably similar to the studies of Wills et al. and Lawrence, which established that pasteurization at 56°C for 15 to 30 min retained higher proportions of immunologic proteins (9,10). It is of interest that the Wills et al. study used an activity assay for determining lysozyme retention, whereas the current study relied on an ELISA method for quantifying this outcome. The latter method is used to quantify individual protein content based on tertiary structure (17), which may account for the considerably lower lysozyme retention observed in this study.
Our findings suggest that temperature, and not the holding time, is critical for the retention of these three proteins. For example, a temperature increase of just 1.7% (from 57°C to 58°C) decreased retention of sIgA, lactoferrin, and lysozyme by 8.5, 34, and 31%, respectively (Fig. 3). In comparison, a similar proportional change in holding time resulted in a 0.68, 0.95, and 0.89% decrease in the retention of sIgA, lactoferrin, and lysozyme, respectively. This illustrates that the importance of accurately monitoring and maintaining pasteurization temperature, because even a small change in temperature can have large adverse effects on the quality of PDHM. It follows that the precision of temperature monitoring will have important implications for milk banks in meeting quality control guidelines for pasteurization conditions, while at the same time retaining protein bioactivity.
Having established that 90% or more of the immunologic proteins were retained at 57°C, it was necessary to determine whether this temperature was also suitable for inactivating a range of common bacteria found in DHM. Although previous studies have assessed the inactivation kinetics of E. coli, S. aureus, and group β-hemolytic Streptococci in human milk during Holder Pasteurization (62.5°C for 30 min; 18), this is the first study that examined B. cereus, S. epidermidis, and E. cloacae at this temperature and all five bacterial species at 57°C. In the food industry, it is well established that the type of food, especially liquid food, can contribute to the effectiveness of pasteurization (19). Therefore, when determining the safety of a pasteurization process for a particular food, it is a common practice that the food of interest is inoculated with a known amount of bacteria and the effectiveness of pasteurization compared against a control. This study used a similar approach, whereby either the human milk or a control medium was inoculated with a final concentration of 105 CFU/mL of an individual species of bacteria, equivalent to the maximum advisable allowable amount in DHM (2–4). In addition, low levels of bacteria were present in some milk samples before inoculation, as evidenced by the higher CFU counts than the number originally inoculated. Pasteurization at either 62.5°C for 20 min or 57°C for 30 min was sufficient to reduce all bacterial species tested by 99.9% (Fig.4). The transfer of M. tuberculosis to the premature infant via DHM remains an important issue in human milk banking, although this risk has never been quantified. Dairy studies have demonstrated that pasteurizing at 62.5°C for 30 min readily inactivates this pathogen, whereas 90 to 95% are inactivated at 57°C for 30 min (20). Therefore, a conflict of interest exists between ensuring the inactivation of rare heat-resistant pathogens and retaining the components that benefit the preterm infant. Thus, current practice (62.5°C for 30 min) may be considered as excessive for pasteurizing the majority of human milk donated to the human milk bank.
The heating profile during pasteurization was also examined in this study, a factor that is highly dependent on pasteurizer design. Compared with the bottle immersion system, the rapid heating (lag time) and cooling of the human milk could be achieved with the experimental system. This ideal heating profile may have contributed to the significant improvement in lysozyme retention, relative to the bottle immersion system. The effect of lag time on protein retention may also be important for Flash Pasteurization (72°C for 15 s). It would be expected from our findings that longer lag times in heating milk from 57°C to 72°C would result in greater protein damage. In addition to the effect on protein retention, lag time is likely to affect the inactivation rates of bacteria. When compared with our findings, previous studies that used the bottle emersion method have demonstrated considerably shorter inactivation times of the bacteria tested in this study (18). This is likely due to the prolonged lag time associated with this method, contributing to bacterial inactivation. In contrast, the extremely short lag time of the experimental pasteurizer is likely to have less of an effect in this regard. Therefore, although a prolonged lag time contributes to bacterial inactivation, it also affects the quality of the final product, and the balance of these desired outcomes must be considered in the design of future human milk pasteurizers.
An advantage of the semiflow-through design of the holding chamber system was the enhanced mixing of the human milk that prevented fat clumping, a problem that is common to both the other pasteurizer designs. Clearly, this is an issue that deserves more attention and could potentially be resolved through future innovations in pasteurizer design and practice. Pasteurizer design is not only important for batch turnaround time but also critical to quality of the final product. As evidenced in this study, improving human milk pasteurization practice through milder conditions, accurate and precise monitoring of pasteurization temperature, and enhancing pasteurizer design to reduce lag time are an achievable means for increasing the quality of PDHM. However, further studies are required to assess the efficacy of pasteurization at 57°C on a wider range of microbial contaminants, including viruses.
Abbreviations
- CFU/ml:
-
colony-forming units/milliliter
- DHM:
-
donor human milk
- MOM:
-
mother's own milk
- PDHM:
-
pasteurized donor human milk
- sIgA:
-
secretory immunoglobulin A
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Acknowledgements
The authors are grateful for the assistance of Mr. Lukas Christen and Mr. Beat Widmer (Carag AG, Switzerland) for providing the technical diagrams of the experimental pasteurizer and to the generosity of the human milk donors that made this research possible.
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Supported by the Rotary Clubs of Thornlie and Belmont (Western Australia), The Women and Infants Research Foundation, The Perron Charitable Trust, and Medela AG (Switzerland).
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Czank, C., Prime, D., Hartmann, B. et al. Retention of the Immunological Proteins of Pasteurized Human Milk in Relation to Pasteurizer Design and Practice. Pediatr Res 66, 374–379 (2009). https://doi.org/10.1203/PDR.0b013e3181b4554a
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DOI: https://doi.org/10.1203/PDR.0b013e3181b4554a
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